Purification and properties of ε-poly-L-lysine-degrading enzyme from Kitasatospora sp.MY5-36

Xiao Hai Feng; Xiao Ying Xu; Zhong Yao; Hong Xu

Purification and properties of ε-poly-L-lysine-degrading enzyme from Kitasatospora sp.MY5-36

Xiao Hai Feng, Xiao Ying Xu, Zhong Yao, Hong Xu

COLLEGE OF FOOD SCIENCE AND LIGHT INDUSTRY

Nanjing Tech University

Research output: Contribution to journal › Article › peer-review

Abstract

A ε-poly-L-lysine-degrading (PLD) enzyme from Kitasatospora sp.MY5-36 was purified and characterized. The enzyme was purified through three steps of anion exchange chromatography including DEAE-Sepharose, Source 15Q and Mono Q. The overall purification multiple was 500 with an enzymatic activity recovery rate of 40.7%. As detected by SDS-PAGE and gel filtration chromatography, the PLD enzyme of this strain was composed of two homogeneous subunits. The molecular weight of subunit and holoenzymes were 43.6 and 87.0 kDa, respectively. Its optimal pH value was 7.0 and the optimal temperature 30°C. The activity of PLD enzyme was kept stable when the enzyme was conserved in the temperature range from 20 to 40°C, however, it declined rapidly in the temperature range from 50 to 60°C. The K_m value was 0.216 mmol/L and the V_max 0.112 mmol/(L·min). The PLD enzyme is a kind of metalloenzymes, and can be activated by Co²⁺ and inhibited by Ca²⁺.

Original language	English
Pages (from-to)	1207-1211
Number of pages	5
Journal	Guocheng Gongcheng Xuebao/The Chinese Journal of Process Engineering
Volume	7
Issue number	6
State	Published - Dec 2007

Keywords

Anion exchange chromatography
Enzymological property
ε-poly-L-lysine-degrading enzyme

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title = "Purification and properties of ε-poly-L-lysine-degrading enzyme from Kitasatospora sp.MY5-36",

abstract = "A ε-poly-L-lysine-degrading (PLD) enzyme from Kitasatospora sp.MY5-36 was purified and characterized. The enzyme was purified through three steps of anion exchange chromatography including DEAE-Sepharose, Source 15Q and Mono Q. The overall purification multiple was 500 with an enzymatic activity recovery rate of 40.7%. As detected by SDS-PAGE and gel filtration chromatography, the PLD enzyme of this strain was composed of two homogeneous subunits. The molecular weight of subunit and holoenzymes were 43.6 and 87.0 kDa, respectively. Its optimal pH value was 7.0 and the optimal temperature 30°C. The activity of PLD enzyme was kept stable when the enzyme was conserved in the temperature range from 20 to 40°C, however, it declined rapidly in the temperature range from 50 to 60°C. The Km value was 0.216 mmol/L and the Vmax 0.112 mmol/(L·min). The PLD enzyme is a kind of metalloenzymes, and can be activated by Co2+ and inhibited by Ca2+.",

keywords = "Anion exchange chromatography, Enzymological property, ε-poly-L-lysine-degrading enzyme",

author = "Feng, {Xiao Hai} and Xu, {Xiao Ying} and Zhong Yao and Hong Xu",

year = "2007",

month = dec,

language = "英语",

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journal = "Guocheng Gongcheng Xuebao/The Chinese Journal of Process Engineering",

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TY - JOUR

T1 - Purification and properties of ε-poly-L-lysine-degrading enzyme from Kitasatospora sp.MY5-36

AU - Feng, Xiao Hai

AU - Xu, Xiao Ying

AU - Yao, Zhong

AU - Xu, Hong

PY - 2007/12

Y1 - 2007/12

N2 - A ε-poly-L-lysine-degrading (PLD) enzyme from Kitasatospora sp.MY5-36 was purified and characterized. The enzyme was purified through three steps of anion exchange chromatography including DEAE-Sepharose, Source 15Q and Mono Q. The overall purification multiple was 500 with an enzymatic activity recovery rate of 40.7%. As detected by SDS-PAGE and gel filtration chromatography, the PLD enzyme of this strain was composed of two homogeneous subunits. The molecular weight of subunit and holoenzymes were 43.6 and 87.0 kDa, respectively. Its optimal pH value was 7.0 and the optimal temperature 30°C. The activity of PLD enzyme was kept stable when the enzyme was conserved in the temperature range from 20 to 40°C, however, it declined rapidly in the temperature range from 50 to 60°C. The Km value was 0.216 mmol/L and the Vmax 0.112 mmol/(L·min). The PLD enzyme is a kind of metalloenzymes, and can be activated by Co2+ and inhibited by Ca2+.

AB - A ε-poly-L-lysine-degrading (PLD) enzyme from Kitasatospora sp.MY5-36 was purified and characterized. The enzyme was purified through three steps of anion exchange chromatography including DEAE-Sepharose, Source 15Q and Mono Q. The overall purification multiple was 500 with an enzymatic activity recovery rate of 40.7%. As detected by SDS-PAGE and gel filtration chromatography, the PLD enzyme of this strain was composed of two homogeneous subunits. The molecular weight of subunit and holoenzymes were 43.6 and 87.0 kDa, respectively. Its optimal pH value was 7.0 and the optimal temperature 30°C. The activity of PLD enzyme was kept stable when the enzyme was conserved in the temperature range from 20 to 40°C, however, it declined rapidly in the temperature range from 50 to 60°C. The Km value was 0.216 mmol/L and the Vmax 0.112 mmol/(L·min). The PLD enzyme is a kind of metalloenzymes, and can be activated by Co2+ and inhibited by Ca2+.

KW - Anion exchange chromatography

KW - Enzymological property

KW - ε-poly-L-lysine-degrading enzyme

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M3 - 文章

AN - SCOPUS:37749044138

SN - 1009-606X

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EP - 1211

JO - Guocheng Gongcheng Xuebao/The Chinese Journal of Process Engineering

JF - Guocheng Gongcheng Xuebao/The Chinese Journal of Process Engineering

IS - 6

ER -

Purification and properties of ε-poly-L-lysine-degrading enzyme from Kitasatospora sp.MY5-36

Abstract

Keywords

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