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镁离子、锰离子和钴离子对酪蛋白激酶2的失活作用。

Casein kinase 2 inactivation by Mg2+, Mn2+ and Co2+ ions.

作者信息

Jiménez J S, Benítez M J, Lechuga C G, Collado M, González-Nicólas J, Moreno F J

机构信息

Departamento de Química Física Aplicada, (UAM), Universidad Autónoma, Madrid, Spain.

出版信息

Mol Cell Biochem. 1995 Nov 8;152(1):1-6. doi: 10.1007/BF01076457.

Abstract

Mg2+ as well as Mn2+, and Co2+, which may substitute Mg2+ in the mental ion requirement of casein kinase 2 (Gatica et al., FEBS Lett: 315:173-173, 1993), have been repeatedly reported to display an optimal concentration at which activity of casein kinase 2 is maximal. As far as we know this intriguing property has always been observed with casein as substrate. This phosphoprotein is not the natural substrate of the enzyme, and it is well known that it binds divalent metal ions, which provoke the aggregation and precipitation of the protein. Since an optimal concentration of metal ion might have a regulatory role, we have examined if it is a consequence of the particular properties of casein, or it is an inherent property of the enzyme, extensive to other substrates. We have used the type II regulatory subunit of protein kinase A which is a physiological substrate of the enzyme, and the peptide RRREEETEEE as a specific substrate. No optimal concentration of Mg2+ is observed when these two substrates are used. The results explain, however, why that optimum is observed with casein. Although low concentration of Mn2+, and Co2+ render about 25% of the maximal activity found with Mg2+, they inactivate the enzyme almost fully at concentrations at which Mg2+ yield the maximal activity.

摘要

镁离子以及锰离子和钴离子,它们在酪蛋白激酶2的金属离子需求中可替代镁离子(加蒂卡等人,《欧洲生物化学学会联合会快报》:315:173 - 173,1993年),已有多次报道显示存在一个最佳浓度,此时酪蛋白激酶2的活性最大。据我们所知,这种有趣的特性一直是在以酪蛋白为底物时观察到的。这种磷蛋白并非该酶的天然底物,而且众所周知它能结合二价金属离子,从而导致蛋白质聚集和沉淀。由于金属离子的最佳浓度可能具有调节作用,我们研究了这是酪蛋白特殊性质的结果,还是该酶的固有性质,并且这种性质是否也适用于其他底物。我们使用了蛋白激酶A的II型调节亚基,它是该酶的一种生理底物,以及肽RRREEETEEE作为特异性底物。当使用这两种底物时,未观察到镁离子的最佳浓度。然而,这些结果解释了为何用酪蛋白时会观察到这种最佳浓度。尽管低浓度的锰离子和钴离子能产生约25%用镁离子时所发现的最大活性,但在镁离子产生最大活性的浓度下,它们几乎能使该酶完全失活。

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