调节蛋白使肝糖原磷酸酶G的催化亚基与糖原分离。
The modulator protein dissociates the catalytic subunit of hepatic protein phosphatase G from glycogen.
作者信息
Bollen M, Stalmans W
机构信息
Afdeling Biochemie, Faculteit Geneeskunde, Katholieke Universiteit Leuven, Belgium.
出版信息
Biochem J. 1988 Mar 15;250(3):659-63. doi: 10.1042/bj2500659.
Abstract
- The phosphorylase phosphatase and glycogen-synthase phosphatase activities associated with the glycogen particles from rat liver were progressively inhibited by incubation with modulator protein. However, the phosphorylase phosphatase activity of the catalytic subunit was entirely recovered after destruction of the modulator and the regulatory subunit(s) by trypsin. 2. Inhibition of protein phosphatase G by modulator was associated with a translocation of the phosphorylase phosphatase activity (measured after incubation with trypsin) from glycogen to the soluble fraction. The degree of inhibition of phosphatase G corresponded closely to the extent to which the phosphorylase phosphatase activity was released from the glycogen particles. Incubation of glycogen-free protein phosphatase G with modulator did not change the affinity of the enzyme for added glycogen, but decreased the amount of phosphatase that could be bound to glycogen. 3. The phosphorylase phosphatase activity that was released from the glycogen particles by modulator migrated on gel filtration as a complex (Mr 106,000) of the catalytic subunit with modulator. Phosphorylase phosphatase activity could be transferred from glycogen-bound protein phosphatase G to modulator that was covalently bound to Sepharose. After elution from the column, the enzyme was identified as the free catalytic subunit (Mr 37,000).
摘要
- 用调节蛋白孵育大鼠肝脏糖原颗粒相关的磷酸化酶磷酸酶和糖原合酶磷酸酶活性会逐渐受到抑制。然而,在用胰蛋白酶破坏调节蛋白和调节亚基后,催化亚基的磷酸化酶磷酸酶活性完全恢复。2. 调节蛋白对蛋白磷酸酶G的抑制作用与磷酸化酶磷酸酶活性(用胰蛋白酶孵育后测定)从糖原向可溶部分的转位有关。磷酸酶G的抑制程度与磷酸化酶磷酸酶活性从糖原颗粒中释放的程度密切相关。用调节蛋白孵育无糖原的蛋白磷酸酶G不会改变该酶对添加糖原的亲和力,但会减少可与糖原结合的磷酸酶量。3. 调节蛋白从糖原颗粒中释放的磷酸化酶磷酸酶活性在凝胶过滤中以催化亚基与调节蛋白的复合物(分子量106,000)形式迁移。磷酸化酶磷酸酶活性可以从与糖原结合的蛋白磷酸酶G转移到与琼脂糖共价结合的调节蛋白上。从柱上洗脱后,该酶被鉴定为游离催化亚基(分子量37,000)。
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本文引用的文献
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