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INDUCTION AND PURIFICATION OF BEAUVERIA-BASSIANA CHITINOLYTIC ENZYMES
被引:24
|
作者
:
HAVUKKALA, I
论文数:
0
引用数:
0
h-index:
0
机构:
KYOTO INST TECHNOL, DEPT CHEM & MAT TECHNOL, BIOCHEM LAB, SAKYO KU, KYOTO 606, JAPAN
KYOTO INST TECHNOL, DEPT CHEM & MAT TECHNOL, BIOCHEM LAB, SAKYO KU, KYOTO 606, JAPAN
HAVUKKALA, I
[
1
]
MITAMURA, C
论文数:
0
引用数:
0
h-index:
0
机构:
KYOTO INST TECHNOL, DEPT CHEM & MAT TECHNOL, BIOCHEM LAB, SAKYO KU, KYOTO 606, JAPAN
KYOTO INST TECHNOL, DEPT CHEM & MAT TECHNOL, BIOCHEM LAB, SAKYO KU, KYOTO 606, JAPAN
MITAMURA, C
[
1
]
HARA, S
论文数:
0
引用数:
0
h-index:
0
机构:
KYOTO INST TECHNOL, DEPT CHEM & MAT TECHNOL, BIOCHEM LAB, SAKYO KU, KYOTO 606, JAPAN
KYOTO INST TECHNOL, DEPT CHEM & MAT TECHNOL, BIOCHEM LAB, SAKYO KU, KYOTO 606, JAPAN
HARA, S
[
1
]
HIRAYAE, K
论文数:
0
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机构:
KYOTO INST TECHNOL, DEPT CHEM & MAT TECHNOL, BIOCHEM LAB, SAKYO KU, KYOTO 606, JAPAN
KYOTO INST TECHNOL, DEPT CHEM & MAT TECHNOL, BIOCHEM LAB, SAKYO KU, KYOTO 606, JAPAN
HIRAYAE, K
[
1
]
NISHIZAWA, Y
论文数:
0
引用数:
0
h-index:
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机构:
KYOTO INST TECHNOL, DEPT CHEM & MAT TECHNOL, BIOCHEM LAB, SAKYO KU, KYOTO 606, JAPAN
KYOTO INST TECHNOL, DEPT CHEM & MAT TECHNOL, BIOCHEM LAB, SAKYO KU, KYOTO 606, JAPAN
NISHIZAWA, Y
[
1
]
HIBI, T
论文数:
0
引用数:
0
h-index:
0
机构:
KYOTO INST TECHNOL, DEPT CHEM & MAT TECHNOL, BIOCHEM LAB, SAKYO KU, KYOTO 606, JAPAN
KYOTO INST TECHNOL, DEPT CHEM & MAT TECHNOL, BIOCHEM LAB, SAKYO KU, KYOTO 606, JAPAN
HIBI, T
[
1
]
机构
:
[1]
KYOTO INST TECHNOL, DEPT CHEM & MAT TECHNOL, BIOCHEM LAB, SAKYO KU, KYOTO 606, JAPAN
来源
:
JOURNAL OF INVERTEBRATE PATHOLOGY
|
1993年
/ 61卷
/ 01期
关键词
:
CHITINOLYTIC ENZYME;
CHITINASE;
N-ACETYLGLUCOSAMINIDASE;
ENZYME INDUCTION;
FUNGUS;
ENTOMOPATHOGEN;
BEAUVERIA-BASSIANA;
PRAYING MANTIS;
STATILIA-MACULATA;
ENZYME PURIFICATION;
D O I
:
10.1006/jipa.1993.1017
中图分类号
:
Q95 [动物学];
学科分类号
:
071002 ;
摘要
:
Chitinolytic enzyme production and induction in an entomopathogenic fungus Beauveria bassiana (an isolate from a praying mantis) was investigated in liquid culture medium. Extracellular chitinolytic proteins could be induced in ca. 20 hr after washed mycelia were transferred to a medium containing colloidal chitin as a sole carbon and nitrogen source. Chitinolytic enzymes were partially purified by ammonium sulfate precipitation followed by gel filtration with a Cellulofine GCL 2000-sf column. Two main degradation activity peaks toward glycolchitin were eluted out. Peak 1 degraded glycolchitin and p-nitrophenyl-β-D-N-acetylglucosaminide (pNP-NAG1), indicating mixed activities of endo- and exochitinase. Peak 2 degraded glycolchitin but not pNP-NAG1, suggesting endochitinase activity. Peak 2 was further purified to homogeneity by ion-exchange chromatography on a Mono Q column and gel filtration through a joint-column of TSKgel G3000SW and G2000SW. The molecular weight of the endochitinase thus purified was estimated to be 45 kDa by SDS-polyacrylamide gel electrophoresis. Copyright © 1993 Academic Press. All rights reserved.
引用
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页码:97 / 102
页数:6
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