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本文引用的文献

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Spontaneous cytosolic calcium pulses in Xenopus melanotrophs are due to calcium influx during phasic increases in the calcium permeability of the cell membrane.
Endocrinology. 1993 May;132(5):2176-83. doi: 10.1210/endo.132.5.8477662.
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The IP3-sensitive calcium store of HIT cells is located in a surface-derived vesicle fraction.人胰岛素瘤细胞(HIT细胞)中对三磷酸肌醇(IP3)敏感的钙储存位于源自表面的囊泡部分。
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Calcium regulation of intracellular pH in pituitary intermediate lobe melanotropes.垂体中间叶促黑素细胞内pH值的钙调节
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A low affinity Ca2+ receptor controls the final steps in peptide secretion from pituitary melanotrophs.一种低亲和力钙离子受体控制垂体黑素细胞刺激素分泌细胞肽分泌的最后步骤。
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Rhythmic exocytosis stimulated by GnRH-induced calcium oscillations in rat gonadotropes.促性腺激素释放激素诱导的大鼠促性腺激素细胞钙振荡刺激的节律性胞吐作用。
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Indications from Mn-quenching of Fura-2 fluorescence in melanotrophs that dopamine and baclofen close Ca channels that are spontaneously open but not those opened by high [K+]O; and that Cd preferentially blocks the latter.
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Exocytosis elicited by action potentials and voltage-clamp calcium currents in individual mouse pancreatic B-cells.单个小鼠胰腺β细胞中动作电位和电压钳钙电流引发的胞吐作用。
J Physiol. 1993 Dec;472:665-88. doi: 10.1113/jphysiol.1993.sp019966.
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A triggered mechanism retrieves membrane in seconds after Ca(2+)-stimulated exocytosis in single pituitary cells.在单个垂体细胞中,一种触发机制在Ca(2+)刺激的胞吐作用后数秒内回收细胞膜。
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Localization of inositol trisphosphate receptor subtype 3 to insulin and somatostatin secretory granules and regulation of expression in islets and insulinoma cells.肌醇三磷酸受体亚型3在胰岛素和生长抑素分泌颗粒中的定位以及在胰岛和胰岛素瘤细胞中的表达调控。
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10
Chromaffin cell cortical actin network dynamics control the size of the release-ready vesicle pool and the initial rate of exocytosis.嗜铬细胞皮质肌动蛋白网络动力学控制着可释放囊泡池的大小和胞吐作用的初始速率。
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多巴胺(D2)受体对大鼠黑素细胞内钙及膜电容变化的调节

Dopamine (D2) receptor regulation of intracellular calcium and membrane capacitance changes in rat melanotrophs.

作者信息

Lee A K

机构信息

University of Washington, Department of Physiology and Biophysics, Seattle 98195, USA.

出版信息

J Physiol. 1996 Sep 15;495 ( Pt 3)(Pt 3):627-40. doi: 10.1113/jphysiol.1996.sp021621.

DOI:10.1113/jphysiol.1996.sp021621
PMID:8887771
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC1160770/
Abstract
  1. Indo-1 microfluorimetry and patch clamp techniques were used to study the decrease in cytosolic [Ca2+] ([Ca2+]i) caused by dopamine (D2) receptor activation and the calcium dependence of membrane capacitance changes in single rat melanotrophs. 2. [Ca2+]i decreased when extracellular calcium was removed or when the calcium channel blockers nickel (2 mM) or cadmium (100 microM) were applied by bath perfusion. 3. Quinpirole, a dopamine (D2) receptor agonist, reduced [Ca2+]i by 55 +/- 9 nM and hyperpolarized membrane potential by 29 +/- 9 mV simultaneously. 4. Quinpirole-induced [Ca2+]i decrease required deactivation of voltage-dependent calcium channels. Voltage clamping the membrane potential at -25 mV prevented the quinpirole-induced [Ca2+]i decrease. Nickel (2 mM) reduced [Ca2+]i without hyperpolarization and precluded additional [Ca2+]i decrease by quinpirole. 5. Membrane capacitance measurement of secretion rates in cells dialysed with buffered calcium solutions showed that secretion began at approximately 400 nM Cai2+. 6. Melanotrophs have IP3-sensitive calcium stores, but no caffeine-sensitive calcium stores. Calcium released from IP3-sensitive calcium stores also stimulated secretion. 7. Secretion in melanotrophs is modulated by protein kinase activators. cAMP (200 microM) enhanced secretion at [Ca2+]i > 1000 nM. Phorbol myristate acetate (PMA; 200 nM) enhanced secretion at [Ca2+]i < 400 nM, but not in the absence of calcium. 8. Dopamine receptor activation can reduce secretion by reducing the calcium influx through calcium channels with hyperpolarization of the membrane potential. However downregulation of either cAMP or protein kinase C activity may also contribute to the decrease in secretion.
摘要
  1. 采用Indo-1微量荧光测定法和膜片钳技术,研究多巴胺(D2)受体激活引起的大鼠单个黑素细胞胞质[Ca2+]([Ca2+]i)降低以及膜电容变化的钙依赖性。2. 去除细胞外钙或通过浴槽灌注施加钙通道阻滞剂镍(2 mM)或镉(100 μM)时,[Ca2+]i降低。3. 多巴胺(D2)受体激动剂喹吡罗使[Ca2+]i降低55±9 nM,同时使膜电位超极化29±9 mV。4. 喹吡罗诱导的[Ca2+]i降低需要电压依赖性钙通道失活。将膜电位钳制在-25 mV可阻止喹吡罗诱导的[Ca2+]i降低。镍(2 mM)降低[Ca2+]i但不引起超极化,并且阻止喹吡罗进一步降低[Ca2+]i。5. 用缓冲钙溶液透析的细胞中,膜电容分泌率测量表明,分泌在约400 nM Cai2+时开始。6. 黑素细胞具有IP3敏感钙库,但没有咖啡因敏感钙库。从IP3敏感钙库释放的钙也刺激分泌。7. 黑素细胞中的分泌受蛋白激酶激活剂调节。cAMP(200 μM)在[Ca²⁺]i>1000 nM时增强分泌。佛波酯肉豆蔻酸酯(PMA;200 nM)在[Ca²⁺]i<400 nM时增强分泌,但在无钙时不增强。8. 多巴胺受体激活可通过减少钙通道的钙内流并使膜电位超极化来减少分泌。然而,cAMP或蛋白激酶C活性的下调也可能导致分泌减少。