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Improved technique for studying ion channels expressed in Xenopus oocytes, including fast superfusion.

机译:用于研究非洲爪蟾卵母细胞中表达的离子通道(包括快速超融合)的改进技术。

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摘要

The study of whole-cell currents from ion channels expressed in Xenopus oocytes with conventional two-electrode voltage clamp has two major limitations. First, the large diameter and spherical geometry of oocytes prevent extremely fast solution changes. Second, the internal medium is not controlled, which limits the experimental versatility of the oocyte expression system. For example, because the internal medium is not controlled, endogenous calcium-activated chloride conductances can contaminate currents measured with channels that are permeable to calcium. We describe a new technique that combines vaseline-gap voltage clamp for oocytes with a fast superfusion system. The vaseline-gap procedure is simplified by having the micropipette that monitors voltage serve a dual role as a perfusion micropipette that controls the internal solution. In addition, the technique provides fast external solution changes that are complete in 30-50 ms. We applied the approach to measure the calcium permeability of a muscle and a neuronal nicotinic acetylcholine receptor. Very fast agonist induced currents were measured without contamination by the secondary activation of calcium-dependent chloride channels.
机译:用常规的两电极电压钳研究非洲爪蟾卵母细胞中表达的离子通道的全细胞电流有两个主要局限性。首先,卵母细胞的大直径和球形几何形状阻止了溶液的极快变化。其次,内部介质不受控制,这限制了卵母细胞表达系统的实验多功能性。例如,由于内部介质不受控制,因此内源性钙激活的氯离子电导会污染通过钙可渗透通道测量的电流。我们描述了一种新技术,该技术结合了具有快速超融合系统的卵母细胞的凡士林间隙电压钳位。通过使监视电压的微量移液器作为控制内部溶液的灌注微量移液器发挥双重作用,从而简化了凡士林间隙程序。此外,该技术还提供快速的外部解决方案更改,这些更改可在30-50毫秒内完成。我们应用该方法来测量肌肉和神经元烟碱型乙酰胆碱受体的钙渗透性。通过钙依赖性氯离子通道的二次活化,测量了非常快的激动剂感应电流,而没有污染。

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