Rapid purification of secretory acid proteinase from Candida albicans and its characterization.
Indian J Biochem Biophys
;
1991 Oct-Dec; 28(5-6): 444-8
Article
in English
| IMSEAR
| ID: sea-28344
ABSTRACT
Secretory acid proteinase from C. albicans was purified from culture supernatant to apparent homogeneity by ion-exchange chromatography. Two isozymes of the proteinase were resolved using a novel chromatofocusing method. The enzyme, which appears to be a glycoprotein, consists of a single polypeptide chain with glutamine at the N-terminus. Its molecular weight is about 45,000 and isoelectric point is pH 4.6. At pH 5, the proteinase is stable at 45 degrees C for at least 15 min. It has a broad substrate specificity. With BSA as a substrate, Km was determined to be 1.6 x 10(-4) M. The enzyme is inhibited by pepstatin and thus is a carboxyl proteinase. It undergoes autocatalytic digestion at or below pH 5.0. The kinetics of induction of proteinase by various proteins are also reported.
Full text:
Available
Index:
IMSEAR (South-East Asia)
Main subject:
Endopeptidases
/
Candida albicans
/
Kinetics
/
Amino Acids
/
Isoelectric Point
/
Isoenzymes
/
Molecular Weight
Language:
English
Journal:
Indian J Biochem Biophys
Year:
1991
Type:
Article
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