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通过网织红细胞裂解物对脊椎动物钙调蛋白进行多次泛素化以及磷酸化酶激酶对钙调蛋白结合的抑制作用。

Multiple ubiquitination of vertebrate calmodulin by reticulocyte lysate and inhibition of calmodulin conjugation by phosphorylase kinase.

作者信息

Ziegenhagen R, Jennissen H P

机构信息

Institut für Physiologie, Ludwig-Maximilians-Universität München.

出版信息

Biol Chem Hoppe Seyler. 1988 Dec;369(12):1317-24. doi: 10.1515/bchm3.1988.369.2.1317.

DOI:10.1515/bchm3.1988.369.2.1317
PMID:2853949
Abstract

Mammalian calmodulin containing trimethyllysine 115 can be covalently coupled to ubiquitin in a Ca2+-dependent manner in the presence of ATP/Mg2+ by reticulocyte lysate. This conjugation reaction can be quantitated in a novel test employing fluphenazine-Sepharose. It is shown that at least 3 ubiquitin molecules can be coupled to calmodulin indicating that more than one lysine residue is involved in the ubiquitination reaction. In addition only the free form of calmodulin can be ubiquitinated. Neither calmodulin bound to phosphorylase kinase as an integral subunit (delta-subunit) nor that bound as a peripheral subunit (delta'-subunit) is ubiquitinated. A total binding of equimolar calmodulin to phosphorylase kinase occurs since the affinity of binding of calmodulin to phosphorylase kinase as integral (KCaMm unknown) or peripheral subunit (KCaMm ca. 30-50nM) is several order of magnitude higher than the corresponding affinity of calmodulin for the ubiquitin-conjugating enzyme (KCaMm ca. 8 microM). We conclude that the "protective" effect of phosphorylase kinase towards calmodulin conjugation is due to a changed conformation of bound calmodulin and/or inacessibility of the ubiquitination sites (e.g. at subunit-subunit interface). Thus Ca2+-dependent ubiquitination only of free calmodulin may provide an efficient scavanging mechanism (with subsequent breakdown) for all free calmodulin in excess of that amount which can be bound by the calmodulin-binding proteins in the cell.

摘要

在ATP/Mg2+存在的情况下,含有三甲基赖氨酸115的哺乳动物钙调蛋白可通过网织红细胞裂解物以Ca2+依赖的方式与泛素共价偶联。这种偶联反应可以在一种使用氟奋乃静-琼脂糖的新型试验中进行定量。结果表明,至少3个泛素分子可以与钙调蛋白偶联,这表明泛素化反应涉及多个赖氨酸残基。此外,只有游离形式的钙调蛋白可以被泛素化。既没有作为完整亚基(δ亚基)与磷酸化酶激酶结合的钙调蛋白,也没有作为外周亚基(δ'亚基)结合的钙调蛋白被泛素化。钙调蛋白与磷酸化酶激酶以等摩尔量完全结合,因为钙调蛋白作为完整亚基(KCaMm未知)或外周亚基(KCaMm约30-50nM)与磷酸化酶激酶结合的亲和力比钙调蛋白对泛素偶联酶的相应亲和力(KCaMm约8μM)高几个数量级。我们得出结论,磷酸化酶激酶对钙调蛋白偶联的“保护”作用是由于结合的钙调蛋白构象改变和/或泛素化位点不可接近(例如在亚基-亚基界面处)。因此,仅游离钙调蛋白的Ca2+依赖性泛素化可能为细胞中所有超过钙调蛋白结合蛋白所能结合量的过量游离钙调蛋白提供一种有效的清除机制(随后分解)。

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