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Calcium-independent increase of transmitter release at frog end-plate by trinitrobenzene sulphonic acid.

机译:三硝基苯磺酸使钙在青蛙端板上释放的钙依赖性增加。

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摘要

1. Application of an amino-residue-modifying reagent, 2,4,6-trinitrobenzene-1-sulphonic acid (TNBS), to the frog neuromuscular junction in high-magnesium Ringer solution rapidly increased both the amplitude of nerve-evoked end-plate potentials (EPPs) and the frequency of miniature end-plate potentials (MEPPs). These showed a similar initial time course and reached a maximum 3-7 min and about 10 min, respectively, after the start of application of 2 mM-TNBS. Then, the EPP amplitude decreased, while the MEPP frequency maintained its plateau value. The increase in transmitter release and the decrease in EPP amplitude by TNBS may have been due to different modes of action. 2. The distribution of MEPP amplitude was unchanged by TNBS treatment. 3. The carbachol-induced postsynaptic potential and the extracellularly recorded presynaptic action current were not affected by TNBS treatment for up to 30 min, indicating that the change in EPP amplitude produced by TNBS was not due to either a postsynaptic effect or a change in action potential at the presynaptic terminal. 4. The frequency of MEPPs was increased by TNBS application even when Ca2+ was omitted from the external Ringer solution or when a specific calcium channel blocker, synthetic omega-conotoxin, was added. This indicates that Ca2+ inflow to the nerve terminal is not necessary for TNBS action. 5. When a calcium chelator, BAPTA, was loaded into the presynaptic nerve terminal, the facilitation of EPPs by trains of nerve stimuli was scarcely observed. This suggested that the cytosolic free Ca2+ in the presynaptic terminal was buffered by BAPTA. Under this condition, the amplitudes of EPPs were increased by TNBS application to the same extent as in the control without BAPTA, but were accompanied by little facilitation. The MEPP frequency was also increased by TNBS to the same extent as in the control. These results suggest strongly that augmentation of transmitter release by TNBS was not due to an increase in cytosolic Ca2+ concentration. 6. These observations suggest that TNBS might react with specific protein(s) on the outer surface of the presynaptic membrane and accelerate the exocytosis of synaptic vesicles.
机译:1.将氨基残基修饰剂2,4,6-三硝基苯-1-磺酸(TNBS)用于高镁林格液中的青蛙神经肌肉接头,可迅速增加神经诱发末端的振幅。极板电位(EPP)和微型终极板电位(MEPP)的频率。这些显示出相似的初始时间过程,并且在开始施用2 mM-TNBS之后分别达到了最长3-7分钟和大约10分钟。然后,EPP振幅下降,而MEPP频率保持其平稳值。 TNBS导致的发射器释放增加和EPP振幅减小可能是由于不同的作用方式引起的。 2. TNBS处理后MEPP振幅的分布没有变化。 3.在长达30分钟的时间里,TNBS处理不会影响卡巴胆碱诱导的突触后电位和细胞外记录的突触前动作电流,这表明TNBS产生的EPP振幅变化不是由于突触后作用或动作变化引起的。突触前末端的电位。 4.即使从外部林格溶液中省略了Ca2 +或添加了特定的钙通道阻滞剂合成的ω-芋螺毒素,通过TNBS施用,MEPP的频率也会增加。这表明TNBS动作不需要Ca2 +流入神经末梢。 5.当将钙螯合剂BAPTA装入突触前神经末梢时,几乎没有观察到一系列神经刺激对EPP的促进作用。这表明突触前末端的胞质游离钙离子被BAPTA缓冲。在这种情况下,TNBS的应用使EPPs的幅度增加到与没有BAPTA的对照相同的程度,但几乎没有促进作用。 TNBS也将MEPP频率提高到与对照组相同的程度。这些结果强烈表明,TNBS增强的递质释放不是由于胞质Ca2 +浓度的增加。 6.这些观察结果表明,TNBS可能与突触前膜外表面的特定蛋白质反应,并加速突触小泡的胞吐作用。

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  • 作者

    Kijima, H; Tanabe, N;

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  • 年度 1988
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