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酸性脱氧核糖核酸酶的蛋白质抑制剂。改进的纯化方法及特性。

Protein inhibitor of acid deoxyribonucleases. Improved purification procedure and properties.

作者信息

Lesca P

出版信息

J Biol Chem. 1976 Jan 10;251(1):116-23.

PMID:396
Abstract

A method is described for the extensive purification of acid deoxyribonuclease (acid DNase) and its specific inhibitor from beef liver, the existence of which had been only supported by indirect evidence. By the use of insolubilized acid deoxyribonuclease, eight other proteins interacting with the enzyme have been detected. One of them (molecular weight, 59,000) was identified as responsible for phosphodiesterase activity which is often a contaminant of DNase preparations. Acid DNase (free of phosphodiesterase) and its inhibitor have been obtained as homogeneous proteins, as determined by sodium dodecyl sulfate-polyacrylamide gel electrophoresis. The molecular weight of acid DNase and its inhibitor are, respectively, 26,500 and 21,500; those of other proteins range from 17,000 to 112,000. The properties of beef liver acid DNase are similar to those described for the enzymes extracted from other sources. The same alteration of DNase kinetics by this inhibitor, as that previously demonstrated with an impure protein has been confirmed; the sigmoidal shape observed at pH 5 for the plot of initial rate versus substrate concentration progressively disappears with increasing pH. We have also demonstrated that RNA, which inhibits the acid DNase through a competitive binding to the catalytic site, is able, like the substrate, to reverse the binding of inhibitor to the enzyme.

摘要

本文描述了一种从牛肉肝脏中大量纯化酸性脱氧核糖核酸酶(酸性DNase)及其特异性抑制剂的方法,此前其存在仅由间接证据支持。通过使用固定化酸性脱氧核糖核酸酶,已检测到与该酶相互作用的其他八种蛋白质。其中一种(分子量59,000)被鉴定为导致磷酸二酯酶活性的原因,磷酸二酯酶活性通常是DNase制剂的污染物。通过十二烷基硫酸钠-聚丙烯酰胺凝胶电泳测定,酸性DNase(不含磷酸二酯酶)及其抑制剂已作为纯蛋白获得。酸性DNase及其抑制剂的分子量分别为26,500和21,500;其他蛋白质的分子量范围为17,000至112,000。牛肉肝脏酸性DNase的性质与从其他来源提取的酶的性质相似。已证实该抑制剂对DNase动力学的改变与先前用不纯蛋白质证明的相同;在pH 5下观察到的初始速率与底物浓度关系图的S形随着pH升高逐渐消失。我们还证明,通过与催化位点竞争性结合来抑制酸性DNase的RNA能够像底物一样逆转抑制剂与酶的结合。

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