Purification and some properties of ε-poly-l-lysine-degrading enzyme from Kitasatospora sp. CCTCC M205012

Xiaohai Feng; Hong Xu; Xiaoying Xu; Jun Yao; Zhong Yao

doi:10.1016/j.procbio.2008.02.009

Purification and some properties of ε-poly-l-lysine-degrading enzyme from Kitasatospora sp. CCTCC M205012

Xiaohai Feng, Hong Xu, Xiaoying Xu, Jun Yao, Zhong Yao

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An ε-poly-l-lysine-degrading enzyme (PLD) from Kitasatospora sp. CCTCC M205012 has been purified to homogeneity by three steps of anion-exchange chromatography including DEAE-Sepharose, Source 15Q and Mono Q, with a 500-fold increase in specific activity and 40.9% yield. The PLD has a molecular mass of approximately 87.0 kDa and consists of two identical subunits with a molecular mass of 43.6 kDa. Electrophoretic shows that the PLD isoelectric point was about 7.2. The optimum temperature and pH for the PLD was 30 °C and 7.0, respectively. The PLD was deactivated by EDTA, which was indicated that the enzyme was a metallo enzyme. The activity of PLD was stimulated by Co²⁺ and inhibited by Ca²⁺ remarkably. The apparent K_m with l-lysyl-p-nitroanilide as substrate was 0.216 mM and the V_max was 0.112 mmol/min mg. The PLD was an exo-type enzyme and monomers of l-lysine were detected during the enzymatic degradation of ε-PL.

源语言	英语
页（从-至）	667-672
页数	6
期刊	Process Biochemistry
卷	43
期	6
DOI	https://doi.org/10.1016/j.procbio.2008.02.009
出版状态	已出版 - 6月 2008

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title = "Purification and some properties of ε-poly-l-lysine-degrading enzyme from Kitasatospora sp. CCTCC M205012",

abstract = "An ε-poly-l-lysine-degrading enzyme (PLD) from Kitasatospora sp. CCTCC M205012 has been purified to homogeneity by three steps of anion-exchange chromatography including DEAE-Sepharose, Source 15Q and Mono Q, with a 500-fold increase in specific activity and 40.9% yield. The PLD has a molecular mass of approximately 87.0 kDa and consists of two identical subunits with a molecular mass of 43.6 kDa. Electrophoretic shows that the PLD isoelectric point was about 7.2. The optimum temperature and pH for the PLD was 30 °C and 7.0, respectively. The PLD was deactivated by EDTA, which was indicated that the enzyme was a metallo enzyme. The activity of PLD was stimulated by Co2+ and inhibited by Ca2+ remarkably. The apparent Km with l-lysyl-p-nitroanilide as substrate was 0.216 mM and the Vmax was 0.112 mmol/min mg. The PLD was an exo-type enzyme and monomers of l-lysine were detected during the enzymatic degradation of ε-PL.",

keywords = "Anion-exchange chromatography, Degradation, Kitasatospora sp. CCTCC M205012, Properties, Purification, ε-Poly-l-lysine-degrading enzyme",

author = "Xiaohai Feng and Hong Xu and Xiaoying Xu and Jun Yao and Zhong Yao",

year = "2008",

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T1 - Purification and some properties of ε-poly-l-lysine-degrading enzyme from Kitasatospora sp. CCTCC M205012

AU - Feng, Xiaohai

AU - Xu, Hong

AU - Xu, Xiaoying

AU - Yao, Jun

AU - Yao, Zhong

PY - 2008/6

Y1 - 2008/6

N2 - An ε-poly-l-lysine-degrading enzyme (PLD) from Kitasatospora sp. CCTCC M205012 has been purified to homogeneity by three steps of anion-exchange chromatography including DEAE-Sepharose, Source 15Q and Mono Q, with a 500-fold increase in specific activity and 40.9% yield. The PLD has a molecular mass of approximately 87.0 kDa and consists of two identical subunits with a molecular mass of 43.6 kDa. Electrophoretic shows that the PLD isoelectric point was about 7.2. The optimum temperature and pH for the PLD was 30 °C and 7.0, respectively. The PLD was deactivated by EDTA, which was indicated that the enzyme was a metallo enzyme. The activity of PLD was stimulated by Co2+ and inhibited by Ca2+ remarkably. The apparent Km with l-lysyl-p-nitroanilide as substrate was 0.216 mM and the Vmax was 0.112 mmol/min mg. The PLD was an exo-type enzyme and monomers of l-lysine were detected during the enzymatic degradation of ε-PL.

AB - An ε-poly-l-lysine-degrading enzyme (PLD) from Kitasatospora sp. CCTCC M205012 has been purified to homogeneity by three steps of anion-exchange chromatography including DEAE-Sepharose, Source 15Q and Mono Q, with a 500-fold increase in specific activity and 40.9% yield. The PLD has a molecular mass of approximately 87.0 kDa and consists of two identical subunits with a molecular mass of 43.6 kDa. Electrophoretic shows that the PLD isoelectric point was about 7.2. The optimum temperature and pH for the PLD was 30 °C and 7.0, respectively. The PLD was deactivated by EDTA, which was indicated that the enzyme was a metallo enzyme. The activity of PLD was stimulated by Co2+ and inhibited by Ca2+ remarkably. The apparent Km with l-lysyl-p-nitroanilide as substrate was 0.216 mM and the Vmax was 0.112 mmol/min mg. The PLD was an exo-type enzyme and monomers of l-lysine were detected during the enzymatic degradation of ε-PL.

KW - Anion-exchange chromatography

KW - Degradation

KW - Kitasatospora sp. CCTCC M205012

KW - Properties

KW - Purification

KW - ε-Poly-l-lysine-degrading enzyme

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Purification and some properties of ε-poly-l-lysine-degrading enzyme from Kitasatospora sp. CCTCC M205012

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