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对池塘蜗牛椎实螺中轴突填充有荧光染料5(6)-羧基荧光素的神经元进行光灭活。

Photoinactivation of neurones axonally filled with the fluorescent dye 5(6)-carboxyfluorescein in the pond snail, Lymnaea stagnalis.

作者信息

Kemenes G, Daykin K, Elliott C J

机构信息

Department of Biology, University of York, Heslington, U.K.

出版信息

J Neurosci Methods. 1991 Oct;39(3):207-16. doi: 10.1016/0165-0270(91)90099-l.

Abstract

We describe a new, simple and reliable technique to fill molluscan neurones from their cut axons with sufficient fluorescent dye for photoinactivation experiments. The fluorescent dye 5(6)-carboxyfluorescein (5-CF) travels quickly up the nerves of the gastropod mollusc, Lymnaea stagnalis into the buccal ganglia and fills the cell bodies in 1-3 h. 5-CF filled neurones can be located in the intact ganglia with low intensity blue light. Impalement shows that they are alive and show normal resting, action and synaptic potentials. Intense laser light (wavelength 442 nm, intensity 0.5 MW.m-2) kills all the 5-CF filled cells in less than 5 min in laboratory reared snails. Unstained neurones are not killed. 5-CF fills neurones quicker than Lucifer yellow (LY) when the dye is applied axonally. Neurones stained with Lucifer yellow do not contain sufficient dye to be killed with 5 min laser illumination, but this irradiation reduces the membrane resistance to less than 25%.

摘要

我们描述了一种新的、简单且可靠的技术,可从其切断的轴突向软体动物神经元中填充足够的荧光染料,用于光灭活实验。荧光染料5(6)-羧基荧光素(5-CF)能迅速沿着腹足纲软体动物椎实螺的神经向上进入口神经节,并在1至3小时内填充细胞体。用低强度蓝光可在完整的神经节中定位5-CF填充的神经元。刺入实验表明它们是活的,且显示出正常的静息电位、动作电位和突触电位。在实验室饲养的蜗牛中,强激光(波长442 nm,强度0.5 MW·m⁻²)可在不到5分钟内杀死所有被5-CF填充的细胞。未染色的神经元不会被杀死。当通过轴突施加染料时,5-CF比荧光黄(LY)更快地填充神经元。用荧光黄染色的神经元所含染料不足以在5分钟激光照射下被杀死,但这种照射会使膜电阻降低至25%以下。

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