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Neurotransmitter modulation of extracellular H+ fluxes from isolated retinal horizontal cells of the skate

机译:滑冰离体视网膜水平细胞对细胞外H +通量的神经递质调节

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摘要

Self-referencing H+-selective microelectrodes were used to measure extracellular H+ fluxes from horizontal cells isolated from the skate retina. A standing H+ flux was detected from quiescent cells, indicating a higher concentration of free hydrogen ions near the extracellular surface of the cell as compared to the surrounding solution. The standing H+ flux was reduced by removal of extracellular sodium or application of 5-(N-ethyl-N-isopropyl) amiloride (EIPA), suggesting activity of a Na+–H+ exchanger. Glutamate decreased H+ flux, lowering the concentration of free hydrogen ions around the cell. AMPA/kainate receptor agonists mimicked the response, and the AMPA/kainate receptor antagonist 6-cyano-7-nitroquinoxaline-2,3-dione (CNQX) eliminated the effects of glutamate and kainate. Metabotropic glutamate agonists were without effect. Glutamate-induced alterations in H+ flux required extracellular calcium, and were abolished when cells were bathed in an alkaline Ringer solution. Increasing intracellular calcium by photolysis of the caged calcium compound NP-EGTA also altered extracellular H+ flux. Immunocytochemical localization of the plasmalemma Ca2+–H+-ATPase (PMCA pump) revealed intense labelling within the outer plexiform layer and on isolated horizontal cells. Our results suggest that glutamate modulation of H+ flux arises from calcium entry into cells with subsequent activation of the plasmalemma Ca2+–H+-ATPase. These neurotransmitter-induced changes in extracellular pH have the potential to play a modulatory role in synaptic processing in the outer retina. However, our findings argue against the hypothesis that hydrogen ions released by horizontal cells normally act as the inhibitory feedback neurotransmitter onto photoreceptor synaptic terminals to create the surround portion of the centre-surround receptive fields of retinal neurones.
机译:自参照H + -选择性微电极用于从滑冰视网膜分离的水平细胞中测量细胞外H + 通量。从静止细胞中检测到固定的H + 通量,表明与周围溶液相比,细胞的细胞外表面附近的游离氢离子浓度更高。除去细胞外钠或应用5-(N-乙基-N-异丙基)阿米洛利(EIPA)可以降低H + 的固定通量,表明Na + –H + 交换器。谷氨酸降低了H + 通量,从而降低了细胞周围游离氢离子的浓度。 AMPA /海藻酸酯受体激动剂模拟了这种反应,而AMPA /海藻酸酯受体拮抗剂6-氰基-7-硝基喹喔啉-2,3-二酮(CNQX)消除了谷氨酸和海藻酸酯的作用。代谢型谷氨酸激动剂没有作用。谷氨酸诱导的H + 通量的变化需要细胞外钙,而当将细胞浸入碱性林格液中时则被废除。通过笼蔽钙化合物NP-EGTA的光解增加细胞内钙,也改变了细胞外H + 通量。质膜Ca 2 + –H + -ATPase(PMCA泵)的免疫细胞化学定位显示在外部丛状层内和孤立的水平细胞上有强烈的标记。我们的研究结果表明,H + 通量的谷氨酸调节起因于钙进入细胞并随后激活质膜Ca 2 + –H + - ATP酶。这些神经递质诱导的细胞外pH的变化可能在外视网膜的突触过程中发挥调节作用。但是,我们的发现与以下假设相抵触:由水平细胞释放的氢离子通常充当感光突触末端上的抑制性反馈神经递质,从而形成视网膜神经元的中心周围感受野的周围部分。

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