SURFACE ACTIVATION OF PRO-CATHEPSIN-L

被引：94

作者：

MASON, RW

MASSEY, SD

机构：

[1] Department of Biochemistry, Virginia Polytechnic Institute, State University, Blacksburg

来源：

BIOCHEMICAL AND BIOPHYSICAL RESEARCH COMMUNICATIONS | 1992年 / 189卷 / 03期

关键词：

D O I：

10.1016/0006-291X(92)90268-P

中图分类号：

Q5 [生物化学]; Q7 [分子生物学];

学科分类号：

071010 ; 081704 ;

摘要：

Pro-cathepsin L is an inactive zymogen that has been shown previously to undergo autolysis at pH 3.0 to give mature forms of the enzyme. We have now been able to demonstrate that this enzyme can undergo activation at pH 5.5 in the presence of negatively charged surfaces. Activation could also be measured at pH 6.0, but no activation occurred at pH 6.5 or higher. The initiation of activation depends upon the presence of a small percentage of active pro-enzyme, and this is then followed by a more rapid activation to give mature forms of the enzyme. No significant intermediate molecular forms of the enzyme were seen. The time taken for processing of the pro-enzyme to single-chain mature enzyme is comparable to that seen in biosynthetic pulse-chase experiments. © 1992.

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页码：1659 / 1666

页数：8

相关论文

共 18 条

[1]

BARRETT AJ, 1981, METHOD ENZYMOL, V80, P535

[2] ANALYSIS OF PROTEIN AND PEPTIDE MIXTURES - EVALUATION OF 3 SODIUM DODECYL SULFATE-POLYACRYLAMIDE GEL-ELECTROPHORESIS BUFFER SYSTEMS [J].

BURY, AF .

JOURNAL OF CHROMATOGRAPHY, 1981, 213 (03) :491-500

[3] NOVEL STRUCTURES CTLA-2-ALPHA AND CTLA-2-BETA EXPRESSED IN MOUSE ACTIVATED T-CELLS AND MAST-CELLS AND HOMOLOGOUS TO CYSTEINE PROTEINASE PROREGIONS [J].

DENIZOT, F ;

BRUNET, JF ;

ROUSTAN, P ;

HARPER, K ;

SUZAN, M ;

LUCIANI, MF ;

MATTEI, MG ;

GOLSTEIN, P .

EUROPEAN JOURNAL OF IMMUNOLOGY, 1989, 19 (04) :631-635

[4] PROCESSING AND LYSOSOMAL LOCALIZATION OF A GLYCOPROTEIN WHOSE SECRETION IS TRANSFORMATION STIMULATED [J].

GAL, S ;

WILLINGHAM, MC ;

GOTTESMAN, MM .

JOURNAL OF CELL BIOLOGY, 1985, 100 (02) :535-544

[5] TRANSFORMATION-DEPENDENT SECRETION OF A LOW-MOLECULAR WEIGHT PROTEIN BY MURINE FIBROBLASTS [J].

GOTTESMAN, MM .

PROCEEDINGS OF THE NATIONAL ACADEMY OF SCIENCES OF THE UNITED STATES OF AMERICA, 1978, 75 (06) :2767-2771

[6] EFFECT OF PROTEINASE-INHIBITORS ON INTRACELLULAR PROCESSING OF CATHEPSIN-B, CATHEPSIN-H AND CATHEPSIN-L IN RAT MACROPHAGES [J].

HARA, K ;

KOMINAMI, E ;

KATUNUMA, N .

FEBS LETTERS, 1988, 231 (01) :229-231

[7] BIOSYNTHESES AND PROCESSING OF LYSOSOMAL CYSTEINE PROTEINASES IN RAT MACROPHAGES [J].

KOMINAMI, E ;

TSUKAHARA, T ;

HARA, K ;

KATUNUMA, N .

FEBS LETTERS, 1988, 231 (01) :225-228

[8] HUMAN-LIVER CATHEPSIN-L [J].

MASON, RW ;

GREEN, GDJ ;

BARRETT, AJ .

BIOCHEMICAL JOURNAL, 1985, 226 (01) :233-241

[9] THE IDENTIFICATION OF THE MAJOR EXCRETED PROTEIN (MEP) FROM A TRANSFORMED MOUSE FIBROBLAST CELL-LINE AS A CATALYTICALLY ACTIVE PRECURSOR FORM OF CATHEPSIN-L [J].

MASON, RW ;

GAL, S ;

GOTTESMAN, MM .

BIOCHEMICAL JOURNAL, 1987, 248 (02) :449-454

[10] THE IDENTIFICATION OF ACTIVE FORMS OF CYSTEINE PROTEINASES IN KIRSTEN-VIRUS-TRANSFORMED MOUSE FIBROBLASTS BY USE OF A SPECIFIC RADIOLABELED INHIBITOR [J].

MASON, RW ;

WILCOX, D ;

WIKSTROM, P ;

SHAW, EN .

BIOCHEMICAL JOURNAL, 1989, 257 (01) :125-129