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本文引用的文献

1
An increase in calcium influx contributes to post-tetanic potentiation at the rat calyx of Held synapse.钙内流增加有助于大鼠海氏壶腹突触的强直后增强。
J Neurophysiol. 2006 Dec;96(6):2868-76. doi: 10.1152/jn.00427.2006. Epub 2006 Aug 9.
2
The decrease in the presynaptic calcium current is a major cause of short-term depression at a calyx-type synapse.突触前钙电流的减少是花萼型突触短期抑制的主要原因。
Neuron. 2005 May 19;46(4):633-45. doi: 10.1016/j.neuron.2005.03.024.
3
Presence and distribution of three calcium binding proteins in projection neurons of the adult rat cochlear nucleus.成年大鼠耳蜗核投射神经元中三种钙结合蛋白的存在及分布
Brain Res. 2005 Mar 28;1039(1-2):63-74. doi: 10.1016/j.brainres.2005.01.057.
4
Developmental changes in parvalbumin regulate presynaptic Ca2+ signaling.小清蛋白的发育变化调节突触前钙离子信号传导。
J Neurosci. 2005 Jan 5;25(1):96-107. doi: 10.1523/JNEUROSCI.3748-04.2005.
5
Developmental expression of the Ca2+-binding proteins calretinin and parvalbumin at the calyx of Held of rats and mice.大鼠和小鼠Held壶腹钙结合蛋白钙视网膜蛋白和小白蛋白的发育表达
Eur J Neurosci. 2004 Sep;20(6):1473-82. doi: 10.1111/j.1460-9568.2004.03604.x.
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Facilitation through buffer saturation: constraints on endogenous buffering properties.通过缓冲饱和实现的促进作用:对内源性缓冲特性的限制
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Mutational analysis of dendritic Ca2+ kinetics in rodent Purkinje cells: role of parvalbumin and calbindin D28k.啮齿动物浦肯野细胞中树突状钙离子动力学的突变分析:小清蛋白和钙结合蛋白D28k的作用
J Physiol. 2003 Aug 15;551(Pt 1):13-32. doi: 10.1113/jphysiol.2002.035824. Epub 2003 Jun 17.
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Ca2+ buffer saturation underlies paired pulse facilitation in calbindin-D28k-containing terminals.钙结合蛋白-D28k阳性终末中,Ca2+ 缓冲饱和是双脉冲易化的基础。
Neuron. 2003 Apr 10;38(1):79-88. doi: 10.1016/s0896-6273(03)00196-x.
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Diffusional mobility of parvalbumin in spiny dendrites of cerebellar Purkinje neurons quantified by fluorescence recovery after photobleaching.通过光漂白后荧光恢复定量测定小脑浦肯野神经元棘状树突中小白蛋白的扩散迁移率。
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10
Calcium dynamics, buffering, and buffer saturation in the boutons of dentate granule-cell axons in the hilus.齿状回颗粒细胞轴突在海马体门区的终扣中的钙动力学、缓冲作用及缓冲饱和度
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小白蛋白是球囊突触小体中的一种可移动的突触前钙缓冲蛋白,它能加速钙离子的衰减和短期易化。

Parvalbumin is a mobile presynaptic Ca2+ buffer in the calyx of Held that accelerates the decay of Ca2+ and short-term facilitation.

作者信息

Müller Martin, Felmy Felix, Schwaller Beat, Schneggenburger Ralf

机构信息

Laboratory of Synaptic Mechanisms, Brain-Mind Institute, Ecole Polytechnique Fédérale de Lausanne, 1015 Lausanne, Switzerland.

出版信息

J Neurosci. 2007 Feb 28;27(9):2261-71. doi: 10.1523/JNEUROSCI.5582-06.2007.

DOI:10.1523/JNEUROSCI.5582-06.2007
PMID:17329423
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC6673482/
Abstract

Presynaptic Ca2+ signaling plays a crucial role in short-term plasticity of synaptic transmission. Here, we studied the role of mobile endogenous presynaptic Ca2+ buffer(s) in modulating paired-pulse facilitation at a large excitatory nerve terminal in the auditory brainstem, the calyx of Held. To do so, we assessed the effect of presynaptic whole-cell recording, which should lead to the diffusional loss of endogenous mobile Ca2+ buffers, on paired-pulse facilitation and on intracellular Ca2+ concentration ([Ca2+]i) transients evoked by action potentials. In unperturbed calyces briefly preloaded with the Ca2+ indicator fura-6F, the [Ca2+]i transient decayed surprisingly fast (tau(fast), approximately 30 ms). Presynaptic whole-cell recordings made without additional Ca2+ buffers slowed the decay kinetics of [Ca2+]i and paired-pulse facilitation (twofold to threefold), but the amplitude of the [Ca2+]i transient was changed only marginally. The fast [Ca2+]i decay was restored by adding the slow Ca2+ buffer EGTA (50-100 microM) or parvalbumin (100 microM), a Ca2+-binding protein with slow Ca2+-binding kinetics, to the presynaptic pipette solution. In contrast, the fast Ca2+ buffer fura-2 strongly reduced the amplitude of the [Ca2+]i transient and slowed its decay, suggesting that the mobile endogenous buffer in calyces of Held has slow, rather than fast, binding kinetics. In parvalbumin knock-out mice, the decay of [Ca2+]i and facilitation was slowed approximately twofold compared with wild-type mice, similar to what is observed during whole-cell recordings in rat calyces of Held. Thus, in young calyces of Held, a mobile Ca2+ buffer with slow binding kinetics, primarily represented by parvalbumin, accelerates the decay of spatially averaged [Ca2+]i and paired-pulse facilitation.

摘要

突触前钙离子信号在突触传递的短期可塑性中起着至关重要的作用。在此,我们研究了可移动内源性突触前钙离子缓冲蛋白在调节听觉脑干中一个大的兴奋性神经末梢(Held壶腹)的双脉冲易化中的作用。为此,我们评估了突触前全细胞记录对双脉冲易化以及动作电位诱发的细胞内钙离子浓度([Ca2+]i)瞬变的影响,突触前全细胞记录会导致内源性可移动钙离子缓冲蛋白的扩散性丢失。在短暂预加载钙离子指示剂fura - 6F的未受干扰的Held壶腹中,[Ca2+]i瞬变衰减惊人地快(快速时间常数tau(fast),约30毫秒)。在不添加额外钙离子缓冲蛋白的情况下进行的突触前全细胞记录减缓了[Ca2+]i的衰减动力学和双脉冲易化(两倍至三倍),但[Ca2+]i瞬变的幅度仅略有变化。通过向突触前移液管溶液中添加慢钙离子缓冲剂乙二醇双乙醚二胺四乙酸(EGTA,50 - 100微摩尔)或小白蛋白(100微摩尔,一种具有慢钙离子结合动力学的钙离子结合蛋白),可恢复快速的[Ca2+]i衰减。相反,快速钙离子缓冲剂fura - 2强烈降低了[Ca2+]i瞬变的幅度并减缓了其衰减,这表明Held壶腹中的可移动内源性缓冲蛋白具有慢而非快的结合动力学。在小白蛋白基因敲除小鼠中,与野生型小鼠相比,[Ca2+]i的衰减和易化减缓了约两倍,这与在大鼠Held壶腹中进行全细胞记录时观察到的情况相似。因此,在幼年Held壶腹中,一种主要由小白蛋白代表的具有慢结合动力学的可移动钙离子缓冲蛋白加速了空间平均[Ca2+]i的衰减和双脉冲易化。