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豆壳过氧化物酶的分离纯化及其性质研究 被引量:45

Purification and Characterization of Soybean Hull Peroxidase
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摘要 从豆壳抽提液经硫酸铵分级沉淀,DEAE-SephadexA-50离子交换层析,ConA-Sepharose4B亲合层析和Bio-GelP-60凝胶过滤,纯化了豆壳过氧化物酶(soybeanhulper-oxidase,ShP).纯化酶的比活力为7077U/mg,在SDS-PAGE上显示出一条蛋白质带.ShP分子量为38000,等电点为3.9;ShP为一含血红素的糖蛋白,含糖量为18.7%,光谱学分析揭示,在406nm处有一典型的Soret带,在510nm和640nm处有特征吸收峰.酶反应的最适pH在4.0附近,最适温度为45℃;在pH2.5~12.0之间较稳定,75℃,保温60min,酶活力残余68%,ShP是一种良好的耐酸碱、耐热过氧化物酶.动力学分析求得ShP的表观Km(愈创木酚)为1.62mmol/L,表现Km(H2O2)为0.34mmol/L.在所测定的化学试剂中,N-3、CN-、Fe3+、Fe2+和Sn2+对酶有较强烈的抑制作用,而重金属离子Ag+、Hg2+、Pb2+、Cu2+。 Soybean hull peroxidase(ShP) was purified to electrophoretic homogeneity by combined consecutive treatments consisting of ammonium sulfate fractionation,ion exchange chromatography on DEAE Sephadex A 50,affinity chromatography on Con A Sepharose 4B and gel filtration on Bio Gel P 60.The specific activity of purified peroxidase was 7077 U/mg.The molecular weight of the enzyme was 38 000 and the isoelectric point was pH 3 9.The enzyme was a glycoprotein(carbohydrate content 18 7%) containing a heme as prosthetic group and showed optimum activity and optimum temperature at pH 4 0 and 45℃,respectively.The enzyme was stable in the pH range from 2 5 to 12 At 90℃,it took 15 min to inactivate 50% of the enzyme.Kinetic studies showed that the reaction catalyzed by the enzyme was in accordance with a Ping Pong mechanism,and a K m for H 2O 2 of 0 34 mmol/L at optimum guaiacol concentration and a K m for guaiacol of 1 62 mmol/L at optimum H 2O 2 concentration were obtained.Peroxidase activity was seriously inhibited by Fe 2+ 、Fe 3+ 、Sn 2+ 、CN - and N 3- ,while no obvious inhibition was observed with Hg 2+ 、Ag +、Pb 2+ 、Cr 3+ 、EDTA and SDS.
出处 《中国生物化学与分子生物学报》 CAS CSCD 1998年第5期577-582,共6页 Chinese Journal of Biochemistry and Molecular Biology
关键词 豆壳过氧化物酶 血红素 纯化与性质 Soybean hull peroxidase,Heme,Purification and characterization
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参考文献2

  • 1马登波,纤维素科学与技术,1996年,4卷,1页
  • 2张龙翔,生化实验方法和技术,1981年,106页

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