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葡萄糖和钾离子对离体大鼠肝脏制剂中糖原磷酸化酶两种形式以及糖原合成酶相互转化的影响。

The effects of glucose and of potassium ions on the interconversion of the two forms of glycogen phosphorylase and of glycogen synthetase in isolated rat liver preparations.

作者信息

Hue L, Bontemps F, Hers H

出版信息

Biochem J. 1975 Oct;152(1):105-14. doi: 10.1042/bj1520105.

Abstract

In the isolated perfused rat liver, increasing glucose concentration from 5.5 to 55 mm in the perfusion medium caused a sequential inactivation of glycogen phosphorylase and activation of glycogen synthetase. The latter change was preceded by a lag period which corresponded to the time required to inactivate the major part of the phosphorylase. 2. The same sequence of events was observed in isolated rat hepatocytes incubated at 37C. In this preparation, the rate of phosphorylase inactivation was greatly increased by increasing the concentration of glucose and/or of K+ ions in the external medium. The same agents also caused the activation of glycogen synthetase, but this effect was secondary to the inactivation of phosphorylase. 3. In both types of preparations, the rate of synthetase activation was modulated by the residual amount of phosphorylase a that remained after the initial phase of rapid inactivation and was independent of glucose concentration. 4. In isolated hepatocytes, the rate of conversion of glucose into glycogen was propotional to the activity of synthetase a in the preparation. This conversion was preceded by a lag period which could be shortened by increasing either glucose or K+ concentration in the medium. The incorporation of labelled glucose into glycogen was simultaneous with a glycogenolytic process which could not be attributed to the activity of phosphorylase a.

摘要

在离体灌注的大鼠肝脏中,将灌注液中的葡萄糖浓度从5.5毫米增加到55毫米会导致糖原磷酸化酶依次失活,糖原合成酶激活。后一种变化之前有一个滞后期,该滞后期与使大部分磷酸化酶失活所需的时间相对应。2. 在37℃孵育的离体大鼠肝细胞中观察到相同的事件序列。在该制备中,通过增加细胞外培养基中葡萄糖和/或钾离子的浓度,磷酸化酶失活的速率大大增加。相同的试剂也会导致糖原合成酶激活,但这种作用是磷酸化酶失活的继发效应。3. 在这两种类型的制备中,合成酶激活的速率由快速失活初始阶段后剩余的磷酸化酶a的残留量调节,且与葡萄糖浓度无关。4. 在离体肝细胞中,葡萄糖转化为糖原的速率与制备中合成酶a的活性成正比。这种转化之前有一个滞后期,通过增加培养基中葡萄糖或钾离子的浓度可以缩短该滞后期。标记葡萄糖掺入糖原的过程与一个糖原分解过程同时发生,该糖原分解过程不能归因于磷酸化酶a的活性。

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