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小鼠肝脏蛋白激酶同工酶对3':5'-环磷酸腺苷的依赖性

Adenosine 3':5'-cyclic monophosphate-dependence of protein kinase isoenzymes from mouse liver.

作者信息

Ueland P M, Doskeland S O

出版信息

Biochem J. 1976 Jul 1;157(1):117-26. doi: 10.1042/bj1570117.

Abstract

Conditions influencing the cyclic AMP-dependence of protein kinase (ATP-protein phosphotransferase, EC 2.7.1.37) during the phosphorylation of histone were studied. Protein kinase from mouse liver cytosol and the two isoenzymes [PK (protein kinase) I and PK II] isolated from the cytosol by DEAE-cellulose chromatography were tested. A relation between concentration of enzyme and cyclic AMP-dependence was observed for both isoenzymes. Moderate dilution of isoenzyme PK II decreased the stimulation of the enzyme by cyclic AMP. Isoenzyme PK I could be diluted 200 times more than isoenzyme PK II before the same decrease in cyclic AMP-dependence appeared. Long-term incubation with high concentrations of histone increased the activity in the absence of cyclic AMP relative to the activity in the presence of the nucleotide. This was more pronounced for isoenzyme PK II than for isoenzyme PK I. The cyclic AMP concentration needed to give half-maximal binding of the nucleotide was the same as the cyclic AMP concentration (Ka) at which the protein kinase had 50% of its maximal activity. The close correlation between binding and activation is also found in the presence of KCl, which increased the apparent activation constant (Ka) for cyclic AMP. With increasing [KCl], a progressively higher proportion of the histone phosphorylation observed in cytosol was due to cyclic AMP-independent (casein) kinases, leading to an overestimation of the degree of activation of the cyclic AMP-dependent protein kinases present. The relative contributions of cyclic AMP-dependent and -independent kinases to histone phosphorylation at different ionic strengths was determined by use of heat-stable inhibitor and phospho-cellulose chromatography.

摘要

研究了在组蛋白磷酸化过程中影响蛋白激酶(ATP - 蛋白质磷酸转移酶,EC 2.7.1.37)环磷酸腺苷(cAMP)依赖性的条件。对来自小鼠肝脏胞质溶胶的蛋白激酶以及通过DEAE - 纤维素色谱法从胞质溶胶中分离出的两种同工酶[PK(蛋白激酶)I和PK II]进行了测试。观察到两种同工酶的酶浓度与cAMP依赖性之间存在关系。同工酶PK II适度稀释会降低cAMP对该酶的刺激作用。在cAMP依赖性出现相同程度降低之前,同工酶PK I的稀释倍数可比同工酶PK II多200倍。与高浓度组蛋白长期孵育会增加在无cAMP情况下相对于存在该核苷酸时的活性。对于同工酶PK II而言,这种情况比同工酶PK I更明显。使核苷酸结合达到半数最大结合所需的cAMP浓度与蛋白激酶具有50%最大活性时的cAMP浓度(Ka)相同。在存在氯化钾(KCl)的情况下也发现结合与激活之间存在密切相关性,KCl增加了cAMP的表观激活常数(Ka)。随着[KCl]的增加,在胞质溶胶中观察到的组蛋白磷酸化中,越来越高比例是由不依赖cAMP的(酪蛋白)激酶引起的,导致对存在的依赖cAMP的蛋白激酶激活程度的高估。通过使用热稳定抑制剂和磷酸纤维素色谱法确定了在不同离子强度下依赖cAMP和不依赖cAMP的激酶对组蛋白磷酸化的相对贡献。

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