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大鼠脑干听觉突触处突触前钙电流的易化作用。

Facilitation of the presynaptic calcium current at an auditory synapse in rat brainstem.

作者信息

Cuttle M F, Tsujimoto T, Forsythe I D, Takahashi T

机构信息

Ion Channel Group, Department of Cell Physiology and Pharmacology, University of Leicester, PO Box 138, Leicester LE1 9HN, UK.

出版信息

J Physiol. 1998 Nov 1;512 ( Pt 3)(Pt 3):723-9. doi: 10.1111/j.1469-7793.1998.723bd.x.

Abstract
  1. The presynaptic calcium current (IpCa) was recorded from the calyx of Held in rat brainstem slices using the whole-cell patch clamp technique. 2. Tetanic activation of IpCa by 1 ms depolarizing voltage steps markedly enhanced the amplitude of IpCa. Using a paired pulse protocol, the second (test) response was facilitated with inter-pulse intervals of less than 100 ms. The facilitation was greater at shorter intervals and was maximal (about 20%) at intervals of 5-10 ms. 3. When the test pulse duration was extended, the facilitation was revealed as an increased rate of IpCa activation. From the current-voltage relationship measured at 1 ms from onset, facilitation could be described by a shift in the half-activation voltage of about -4 mV. 4. IpCa facilitation was not attenuated when guanosine-5'-O-(3-thiotriphosphate) (GTPgammaS) or guanosine-5'-O-(2-thiodiphosphate) (GDPbetaS) was included in the patch pipette, suggesting that G-proteins are not involved in this phenomenon. 5. On reducing [Ca2+]o, the magnitude of facilitation diminished proportionally to the amplitude of IpCa. Replacement of [Ca2+]o by Ba2+ or Na+, or buffering of [Ca2+]i with EGTA or BAPTA attenuated IpCa facilitation. 6. We conclude that repetitive presynaptic activity can facilitate the presynaptic Ca2+ current through a Ca2+-dependent mechanism. This mechanism would be complementary to the action of residual Ca2+ on the exocytotic machinery in producing activity-dependent facilitation of synaptic responses.
摘要
  1. 使用全细胞膜片钳技术,在大鼠脑干切片的Held壶腹记录突触前钙电流(IpCa)。2. 通过1 ms去极化电压阶跃对IpCa进行强直激活,显著增强了IpCa的幅度。采用双脉冲方案,当脉冲间隔小于100 ms时,第二个(测试)反应得到易化。间隔越短,易化作用越强,在5 - 10 ms间隔时达到最大(约20%)。3. 当测试脉冲持续时间延长时,易化表现为IpCa激活速率增加。从起始后1 ms测量的电流 - 电压关系来看,易化作用可通过半激活电压约 - 4 mV的偏移来描述。4. 当膜片电极内加入鸟苷 - 5'-O -(3 - 硫代三磷酸)(GTPγS)或鸟苷 - 5'-O -(2 - 硫代二磷酸)(GDPβS)时,IpCa易化作用并未减弱,这表明G蛋白不参与此现象。5. 降低细胞外钙浓度([Ca2+]o)时,易化幅度与IpCa幅度成比例减小。用Ba2+或Na+替代[Ca2+]o,或用乙二醇双(2 - 氨基乙醚)四乙酸(EGTA)或1,2 - 双(2 - 氨基苯氧基)乙烷 - N,N,N',N'-四乙酸(BAPTA)缓冲细胞内钙浓度([Ca2+]i),均可减弱IpCa易化作用。6. 我们得出结论,重复性突触前活动可通过钙依赖机制促进突触前钙电流。该机制在产生依赖活动的突触反应易化过程中,与残余钙对外排机制的作用互补。

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