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发育中海鞘肌肉卵裂球中电压依赖性Ca2+通道与兰尼碱受体之间的交叉偶联。

Cross-coupling between voltage-dependent Ca2+ channels and ryanodine receptors in developing ascidian muscle blastomeres.

作者信息

Nakajo K, Chen L, Okamura Y

机构信息

Department of Life Sciences, Graduate Program in Interdisciplinary Sciences, The University of Tokyo, 3-8-1 Komaba, Meguro-ku, Tokyo 153-0041, Japan.

出版信息

J Physiol. 1999 Mar 15;515 ( Pt 3)(Pt 3):695-710. doi: 10.1111/j.1469-7793.1999.695ab.x.

Abstract
  1. Ascidian blastomeres of muscle lineage express voltage-dependent calcium channels (VDCCs) despite isolation and cleavage arrest. Taking advantage of these large developing cells, developmental changes in functional relations between VDCC currents and intracellular Ca2+ stores were studied. 2. Inactivation of ascidian VDCCs is Ca2+ dependent, as demonstrated by two pieces of evidence: (1) a bell-shaped relationship between prepulse voltage and amplitude during the test pulse in Ca2+, but not in Ba2+, and (2) the decay kinetics of Ca2+ currents (ICa) obtained as the size of tail currents. 3. During replacement in the external solution of Ca2+ with Ba2+, the inward current appeared biphasic: it showed rapid decay followed by recovery and slow decay. This current profile was most evident in the mixed bath solution (2 % Ca2+ and 98 % Ba2+, abbreviated to '2Ca/98Ba'). 4. The biphasic profile of I2Ca/98Ba was significantly attenuated in caffeine and in ryanodine, indicating that Ca2+ release is involved in shaping the current kinetics of VDCCs. After washing out the caffeine, the biphasic pattern was reproducibly restored by depolarizing the membrane in calcium-rich solution, which is expected to refill the internal Ca2+ stores. 5. The inhibitors of endoplasmic reticulum (ER) Ca2+-ATPase (SERCAs) cyclopiazonic acid (CPA) and thapsigargin facilitated elimination of the biphasic profile with repetitive depolarization. 6. At a stage earlier than 36 h after fertilization, the biphasic profile of I2Ca/98Ba was not observed. However, caffeine induced a remarkable decrease in the amplitude of I2Ca/98Ba and this suppression was blocked by microinjection of the Ca2+ chelator BAPTA, showing the presence of caffeine-sensitive Ca2+ stores at this stage. 7. Electron microscopic observation shows that sarcoplasmic membranes (SR) arrange closer to the sarcolemma with maturation, suggesting that the formation of the ultrastructural machinery underlies development of the cross-coupling between VDCCs and Ca2+ stores.
摘要
  1. 尽管被分离并停止分裂,但肌肉谱系的海鞘卵裂球仍表达电压依赖性钙通道(VDCCs)。利用这些正在发育的大细胞,研究了VDCC电流与细胞内钙库之间功能关系的发育变化。2. 海鞘VDCCs的失活是钙依赖性的,有两条证据证明:(1)在钙离子中测试脉冲期间预脉冲电压与幅度之间呈钟形关系,而在钡离子中则不然;(2)作为尾电流大小获得的钙电流(ICa)的衰减动力学。3. 在外部溶液中用钡离子替代钙离子期间,内向电流呈双相:它显示出快速衰减,随后恢复并缓慢衰减。这种电流特征在混合浴溶液(2%钙离子和98%钡离子,简称为“2Ca/98Ba”)中最为明显。4. I2Ca/98Ba的双相特征在咖啡因和ryanodine中显著减弱,表明钙释放参与塑造VDCCs的电流动力学。洗去咖啡因后,通过在富含钙的溶液中使膜去极化可重现地恢复双相模式,这有望重新填充内部钙库。5. 内质网(ER)钙ATP酶(SERCAs)的抑制剂环匹阿尼酸(CPA)和毒胡萝卜素通过重复去极化促进双相特征的消除。6. 在受精后36小时之前的阶段,未观察到I2Ca/98Ba的双相特征。然而,咖啡因导致I2Ca/98Ba的幅度显著降低,并且这种抑制被微量注射钙螯合剂BAPTA阻断,表明在此阶段存在对咖啡因敏感的钙库。7. 电子显微镜观察表明,肌浆膜(SR)随着成熟而更靠近肌膜排列,表明超微结构机制的形成是VDCCs与钙库之间交叉偶联发育的基础。

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