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GABAB receptor- and metabotropic glutamate receptor-dependent cooperative long-term potentiation of rat hippocampal GABAA synaptic transmission

机译:大鼠海马GABAA突触传递的GABAB受体和代谢型谷氨酸受体依赖性协同长期增强

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摘要

Repetitive stimulation of Schaffer collaterals induces activity-dependent changes in the strength of polysynaptic inhibitory postsynaptic potentials (IPSPs) in hippocampal CA1 pyramidal neurons that are dependent on stimulation parameters. In the present study, we investigated the effects of two stimulation patterns, theta-burst stimulation (TBS) and 100 Hz tetani, on pharmacologically isolated monosynaptic GABAergic responses in adult CA1 pyramidal cells. Tetanization with 100 Hz trains transiently depressed both early and late IPSPs, whereas TBS induced long-term potentiation (LTP) of early IPSPs that lasted at least 30 min. Mechanisms mediating this TBS-induced potentiation were examined using whole-cell recordings. The paired-pulse ratio of monosynaptic inhibitory postsynaptic currents (IPSCs) was not affected during LTP, suggesting that presynaptic changes in GABA release are not involved in the potentiation. Bath application of the GABAB receptor antagonist or the group I/II metabotropic glutamate receptor antagonist E4-CPG inhibited IPSC potentiation. Preventing postsynaptic G-protein activation or Ca2+ rise by postsynaptic injection of GDP-β-S or BAPTA, respectively, abolished LTP, indicating a G-protein- and Ca2+-dependent induction in this LTP. Finally during paired-recordings, activation of individual interneurons by intracellular TBS elicited solely short-term increases in average unitary IPSCs in pyramidal cells. These results indicate that a stimulation paradigm mimicking the endogenous theta rhythm activates cooperative postsynaptic mechanisms dependent on GABABR, mGluR, G-proteins and intracellular Ca2+, which lead to a sustained potentiation of GABAA synaptic transmission in pyramidal cells. GABAergic synapses may therefore contribute to functional synaptic plasticity in adult hippocampus.
机译:重复刺激Schaffer侧支会诱导依赖于刺激参数的海马CA1锥体神经元多突触抑制突触后电位(IPSPs)强度的活动依赖性变化。在本研究中,我们调查了成年CA1锥体细胞中药理学上分离的单突触GABA能反应的两种刺激模式,即theta-burst刺激(TBS)和100 Hz的邻苯二酚。 100 Hz训练的钛化作用会暂时抑制早期和晚期IPSP,而TBS会诱导持续至少30分钟的早期IPSP的长期增强(LTP)。使用全细胞记录检查了介导这种TBS诱导的增强作用的机制。 LTP期间单突触抑制性突触后电流(IPSCs)的成对脉冲比率不受影响,这表明增强电位不涉及突触前GABA释放的变化。 GABAB受体拮抗剂或I / II组代谢型谷氨酸受体拮抗剂E4-CPG的沐浴应用可抑制IPSC增强。分别通过突触后注射GDP-β-S或BAPTA防止突触后G蛋白活化或Ca 2 + 升高,从而消除了LTP,表明G蛋白和Ca 2 + 依赖性诱导。最后,在配对记录期间,细胞内TBS对单个中间神经的激活仅引起锥体细胞中平均单位IPSC的短期增加。这些结果表明,模仿内源性θ节律的刺激范式激活了依赖于GABABR,mGluR,G蛋白和细胞内Ca 2 + 的协同突触后机制,从而导致了金字塔形区域中GABAA突触传递的持续增强。细胞。因此,GABA能突触可能有助于成年海马的功能性突触可塑性。

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