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Human placental diamine oxidase. Improved purification and characterization of a copper- and manganese-containing amine oxidase with novel substrate specificity.

机译:人胎盘二胺氧化酶。具有新型底物特异性的含铜和锰的胺氧化酶的改进的纯化和表征。

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摘要

1. Isoelectric focusing studies of human placental diamine oxidase showed the pI value of the active enzyme to be 6.5. This information was used in modifying the enzyme purification by incorporating column chromatography on DEAE-Sephadex with ionic strength and pH gradient elution and this, together with affinity chromatography on concanavalin A--Sepharose, gave a highly purified preparation, with a specific activity of 7.0 units/mg. 2. The enzyme gave the expected stoicheiometry with p-dimethylaminomethylbenzylamine as substrate (Keq. 2700) and also oxidized [8-arginine]vasopressin, [8-lysine]vasopressin, collagen and tropocollagen. Polyacrylamide gel slices showed identical migration of diamine-oxidizing and [8-lysine]vasopressin-oxidizing activity. 3. The molecular weight, determined by ultracentrifugation, sodium dodecyl sulphate/polyacrylamide-gel electrophoresis, variable polyacrylamide-gel electrophoresis and Sephadex G-200 column chromatography, was estimated to be approx. 70000. 4. E.s.r. spectroscopy showed that copper and manganese were present in the purified enzyme. This result was confirmed by atomic absorption spectroscopy, which indicated a stoicheiometry for copper and manganese of approx. 1.0 and 1.2g-atom respectively/70000mol.wt. unit. 5. The e.s.r. spectral intensity did not decrease nor did the spectral line shape change when excess of p-dimethylaminomethylbenzylamine was added to the enzyme. 6. Addition of K13CN to the enzyme eliminated the copper e.s.r. signal without affecting the manganese signal. 7. The placental enzyme therefore appears to differ from other amine oxidases in terms of its metal cofactor requirement, molecular weight and substrate specificity, and possible roles in vivo for this enzyme are discussed.
机译:1.人胎盘二胺氧化酶的等电聚焦研究表明,该活性酶的pI值为6.5。该信息通过结合DEAE-Sephadex上的柱层析(具有离子强度和pH梯度洗脱)用于修饰酶的纯化,并与伴刀豆球蛋白A-Sepharose上的亲和层析相结合,制得了高纯度的制剂,比活性为7.0单位/毫克2.该酶以对二甲基氨基甲基苄胺为底物(Keq。2700),并且还氧化了[8-精氨酸]血管加压素,[8-赖氨酸]血管加压素,胶原蛋白和原胶原,提供了预期的化学计量。聚丙烯酰胺凝胶片显示出相同的二胺氧化和[8-赖氨酸]加压素氧化活性迁移。 3.通过超速离心,十二烷基硫酸钠/聚丙烯酰胺-凝胶电泳,可变聚丙烯酰胺-凝胶电泳和Sephadex G-200柱色谱法测定的分子量估计为约3。 70000。4. E.s.r.光谱显示纯化的酶中存在铜和锰。原子吸收光谱法证实了该结果,该原子吸收光谱法表明铜和锰的化学计量比约为1。 1.0和1.2g原子分别/70000mol.wt。单元。 5. e.s.r.当将过量的对二甲基氨基甲基苄胺添加到酶中时,光谱强度没有降低,谱线形状也没有改变。 6.在酶中加入K 13 CN消除了铜的e.s.r。信号不会影响锰信号。 7.因此,胎盘酶在金属辅因子的需要量,分子量和底物特异性方面似乎与其他胺氧化酶不同,并讨论了该酶在体内的可能作用。

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