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Pre- and postsynaptic whole-cell recordings in the medial nucleus of the trapezoid body of the rat.

机译:大鼠梯形体内侧核中突触前和突触后全细胞记录。

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摘要

1. Simultaneous whole-cell recordings in a rat brain slice preparation are described from presynaptic terminals (calyces of Held) and postsynaptic somata which form an axosomatic synapse in the medial nucleus of the trapezoid body (MNTB). 2. Presynaptic action potentials evoked suprathreshold excitatory postsynaptic potentials (EPSPs). The minimum synaptic delay was around 0.4 ms at 36 degrees C and 0.9 ms at 23-24 degrees C. The amplitude of the L-alpha-amino-3-hydroxy-5-methyl-4-isoxazolepropionate (AMPA) receptor-mediated component of the excitatory postsynaptic currents (EPSCs) was 2-13 nA (at -80 mV). 3. Current-voltage relations showed that presynaptic Ca2+ channels were of the high voltage-activated type. 4. A single action potential evoked a presynaptic fluorescence transient that decayed with a time constant of 0.3-0.7 s, depending on the concentration (60-200 microM) of the Ca2+ indicator Calcium Green-5N (CG-5N). The peak amplitude of the [Ca2+]i transient was severalfold larger in the terminal than in the preterminal axon. 5. EPSC peak amplitudes were stable for more than 30 min after establishing the whole-cell configuration in the presynaptic terminal when the pipette contained 50 microM BAPTA. In contrast, with 1 mM BAPTA, peak amplitudes of EPSCs were reduced to one-third. 6. Trains of presynaptic action potentials evoked EPSCs with progressively smaller amplitudes. Little change was observed in the depression when the terminals were dialysed with 50 microM BAPTA, whereas depression was reduced with 1 mM BAPTA. 7. In low (1 mM) [Ca2+]o, facilitation instead of depression of EPSCs was observed. 8. The effects of presynaptic BAPTA suggest that the endogenous mobile Ca2+ buffer capacity of giant presynaptic terminals in the MNTB is lower than in other terminals of fast transmitting synapses.
机译:1.从突触前的末端(Held的大动脉)和突触后的躯体(在梯形体(MNTB)的内侧核中形成无囊突触)描述了大鼠脑切片制备过程中同时进行的全细胞记录。 2.突触前动作电位诱发阈上兴奋性突触后电位(EPSPs)。最小突触延迟在36摄氏度时约为0.4毫秒,在23-24摄氏度时约为0.9毫秒。L-α-氨基-3-羟基-5-羟基-5-甲基-4-异恶唑丙酸酯(AMPA)受体介导的成分的振幅兴奋性突触后电流(EPSC)的2-13 nA(在-80 mV时)。 3.电流-电压关系表明突触前Ca 2+通道是高电压激活型的。 4.单个动作电位引起突触前荧光瞬变,其衰减时间为0.3-0.7 s,具体取决于Ca2 +指示剂钙绿5N(CG-5N)的浓度(60-200 microM)。在末端,[Ca2 +] i瞬态的峰值幅度比末端前轴突大几倍。 5.当移液管中含有50 microM BAPTA时,在突触前末端建立全细胞构型后,EPSC峰值幅度稳定超过30分钟。相反,使用1 mM BAPTA时,EPSC的峰值幅度降低到三分之一。 6.突触前动作电位的列车诱发幅度逐渐减小的EPSC。当终端用50 microM BAPTA透析时,在抑郁症中观察到的变化很小,而使用1 mM BAPTA透析则降低了抑郁症。 7.在低(1 mM)[Ca2 +] o下,观察到促进作用而不是EPSC抑制。 8.突触前BAPTA的影响表明,MNTB中巨大的突触前末端的内源性移动Ca2 +缓冲能力低于快速传递突触的其他末端。

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