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膜联蛋白I氨基末端结构域在调节其与膜相互作用中的作用:氨基末端截短及磷酸化位点诱变的影响

Role of the amino-terminal domain in regulating interactions of annexin I with membranes: effects of amino-terminal truncation and mutagenesis of the phosphorylation sites.

作者信息

Wang W, Creutz C E

机构信息

Department of Microbiology, University of Virginia School of Medicine, Charlottesville 22908.

出版信息

Biochemistry. 1994 Jan 11;33(1):275-82. doi: 10.1021/bi00167a036.

DOI:10.1021/bi00167a036
PMID:8286349
Abstract

Phosphorylation of the N-terminal tail by protein kinase C strongly inhibits the ability of bovine or human annexin I to aggregate chromaffin granules by increasing the calcium requirement 4-fold (Wang, W., & Creutz, C. E. (1992) Biochemistry 31, 9934-9936). In the present study three forms of human annexin I truncated in the amino terminus at residue Trp-12, Lys-26, or Lys-29 exhibit dramatic differences in their sensitivities to calcium in a chromaffin granule aggregation assay, while the Ca2+max values for binding of the truncated proteins to granule membranes are similar. Cleavage at Trp-12 causes a 3-fold decrease in calcium sensitivity in the membrane aggregation assay, while cleavage at Lys-26 causes a 4-fold enhancement of calcium sensitivity. In contrast, cleavage at Lys-29 results in virtually no change in calcium sensitivity. Mutagenic substitution with negatively charged amino acids of Ser-27, a site for phosphorylation by protein kinase C, or Tyr-21, a site for phosphorylation by the epidermal growth factor receptor kinase, mimics the inhibition of granule-aggregating activity seen with phosphorylation by protein kinase C. When bovine chromaffin cells are stimulated to secrete by nicotine, annexin I is phosphorylated in the amino terminus. Thr-24 and Ser-28, which are sites for phosphorylation by protein kinase C in vitro, are two of the sites phosphorylated in vivo in stimulated chromaffin cells. These data demonstrate that the ability of annexin I to promote membrane aggregation is highly sensitive to changes in the structure of the N-terminal domain of the protein.(ABSTRACT TRUNCATED AT 250 WORDS)

摘要

蛋白激酶C对N端尾部的磷酸化通过将钙需求提高4倍,强烈抑制牛或人膜联蛋白I聚集嗜铬颗粒的能力(Wang, W., & Creutz, C. E. (1992) Biochemistry 31, 9934 - 9936)。在本研究中,在氨基酸末端Trp - 12、Lys - 26或Lys - 29处截短的三种人膜联蛋白I形式,在嗜铬颗粒聚集试验中对钙的敏感性表现出显著差异,而截短蛋白与颗粒膜结合的Ca2 + max值相似。在Trp - 12处切割导致膜聚集试验中钙敏感性降低3倍,而在Lys - 26处切割导致钙敏感性提高4倍。相比之下,在Lys - 29处切割几乎不会导致钙敏感性变化。用带负电荷的氨基酸对蛋白激酶C磷酸化位点Ser - 27或表皮生长因子受体激酶磷酸化位点Tyr - 21进行诱变取代,模拟了蛋白激酶C磷酸化对颗粒聚集活性的抑制作用。当用尼古丁刺激牛嗜铬细胞分泌时,膜联蛋白I在氨基末端被磷酸化。Thr - 24和Ser - 28是体外蛋白激酶C的磷酸化位点,是受刺激的嗜铬细胞体内磷酸化的两个位点。这些数据表明,膜联蛋白I促进膜聚集的能力对蛋白质N端结构域的变化高度敏感。(摘要截短于250字)

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