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钙调蛋白依赖钙离子的核内积聚机制。

Mechanism of Ca2+-dependent nuclear accumulation of calmodulin.

作者信息

Liao B, Paschal B M, Luby-Phelps K

机构信息

Department of Physiology, University of Texas Southwestern Medical Center at Dallas, TX 75235, USA.

出版信息

Proc Natl Acad Sci U S A. 1999 May 25;96(11):6217-22. doi: 10.1073/pnas.96.11.6217.

Abstract

The intracellular Ca2+ receptor calmodulin (CaM) coordinates responses to extracellular stimuli by modulating the activities of its various binding proteins. Recent reports suggest that, in addition to its familiar functions in the cytoplasm, CaM may be directly involved in rapid signaling between cytoplasm and nucleus. Here we show that Ca2+-dependent nuclear accumulation of CaM can be reconstituted in permeabilized cells. Accumulation was blocked by M13, a CaM antagonist peptide, but did not require cytosolic factors or an ATP regenerating system. Ca2+-dependent influx of CaM into nuclei was not blocked by inhibitors of nuclear localization signal-mediated nuclear import in either permeabilized or intact cells. Fluorescence recovery after photobleaching studies of CaM in intact cells showed that influx is a first-order process with a rate constant similar to that of a freely diffusible control molecule (20-kDa dextran). Studies of CaM efflux from preloaded nuclei in permeablized cells revealed the existence of three classes of nuclear binding sites that are distinguished by their Ca2+-dependence and affinity. At high [Ca2+], efflux was enhanced by addition of a high affinity CaM-binding protein outside the nucleus. These data suggest that CaM diffuses freely through nuclear pores and that CaM-binding proteins in the nucleus act as a sink for Ca2+-CaM, resulting in accumulation of CaM in the nucleus on elevation of intracellular free Ca2+.

摘要

细胞内钙离子受体钙调蛋白(CaM)通过调节其各种结合蛋白的活性来协调对细胞外刺激的反应。最近的报道表明,除了在细胞质中常见的功能外,CaM可能直接参与细胞质与细胞核之间的快速信号传导。在这里,我们表明,在透化细胞中可以重建CaM的钙离子依赖性核积累。积累被CaM拮抗剂肽M13阻断,但不需要胞质因子或ATP再生系统。在透化细胞或完整细胞中,钙离子依赖性的CaM流入细胞核不受核定位信号介导的核输入抑制剂的阻断。对完整细胞中CaM进行光漂白后的荧光恢复研究表明,流入是一个一级过程,其速率常数与自由扩散的对照分子(20 kDa葡聚糖)相似。对透化细胞中预加载细胞核的CaM流出研究揭示了三类核结合位点的存在,它们通过其钙离子依赖性和亲和力来区分。在高钙离子浓度下,通过在细胞核外添加高亲和力的CaM结合蛋白可增强流出。这些数据表明,CaM可自由通过核孔扩散,细胞核中的CaM结合蛋白充当钙离子-CaM的汇,导致细胞内游离钙离子升高时CaM在细胞核中积累。

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