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从大鼠脑中快速纯化蛋白激酶C。一种采用鱼精蛋白-琼脂糖亲和柱层析的新方法。

Rapid purification of protein kinase C from rat brain. A novel method employing protamine-agarose affinity column chromatography.

作者信息

Wooten M W, Vandenplas M, Nel A E

出版信息

Eur J Biochem. 1987 Apr 15;164(2):461-7. doi: 10.1111/j.1432-1033.1987.tb11079.x.

Abstract

We describe a rapid purification of protein kinase C from rat brain cytosol employing a specific substrate, protamine-coupled to agarose. Sequential chromatography on DEAE-Sephacel, phenyl-Sepharose CL-4B, and protamine-agarose columns resulted in a 1,500-fold purification of protein kinase C. SDS-PAGE analysis of the purified enzyme resolved a doublet protein of 77-80 kDa. This doublet was recognized by a polyclonal antiserum against protein kinase C. Proteolytic digestion of each protein band generated similar peptide fragments. The underlying principle of the protamine sulfate purification method was also clarified. Protamine can serve as a Ca2+/phospholipid-independent substrate. We demonstrate phosphorylation of protamine on the column; phosphorylated protamine did not bind the enzyme with the same affinity and this covalent modification was most probably responsible for releasing the bound enzyme from the column after addition of Mg2+ and ATP. The C kinase inhibitor, H7, inhibits protamine phosphorylation in a dose-dependent fashion but does not prevent binding of the enzyme to a protamine-agarose column. We therefore conclude that protamine interacts with the active center of the enzyme enabling it to be phosphorylated, upon which it loses its binding affinity for C kinase.

摘要

我们描述了一种从大鼠脑细胞质溶胶中快速纯化蛋白激酶C的方法,该方法使用与琼脂糖偶联的特异性底物鱼精蛋白。依次通过DEAE-葡聚糖凝胶、苯基-琼脂糖凝胶CL-4B和鱼精蛋白-琼脂糖柱进行层析,使蛋白激酶C得到了1500倍的纯化。对纯化后的酶进行SDS-PAGE分析,得到了一条77 - 80 kDa的双峰蛋白条带。该双峰被抗蛋白激酶C的多克隆抗血清识别。对每个蛋白条带进行蛋白酶消化产生了相似的肽片段。硫酸鱼精蛋白纯化方法的基本原理也得到了阐明。鱼精蛋白可作为一种不依赖Ca2+/磷脂的底物。我们证明了柱上鱼精蛋白的磷酸化;磷酸化的鱼精蛋白与酶的结合亲和力不同,这种共价修饰很可能是在加入Mg2+和ATP后使结合的酶从柱上释放的原因。C激酶抑制剂H7以剂量依赖的方式抑制鱼精蛋白的磷酸化,但不阻止酶与鱼精蛋白-琼脂糖柱的结合。因此,我们得出结论,鱼精蛋白与酶的活性中心相互作用,使其能够被磷酸化,磷酸化后它对C激酶的结合亲和力丧失。

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