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[蜗牛巨型神经元的细胞内灌注]

[Intracellular perfusion of the giant neurons of snails].

作者信息

Kryshtal' O A, Pidoplichko V I

出版信息

Neirofiziologiia. 1975;7(3):327-9.

PMID:1153033
Abstract

The method is developed to perform intracellular perfusion of isolated Helix pomatia neurons. The cell is put under hydrostatic pressure into a pore in the plastic film separting the experimental chamber in two compartmentsmthe lower compartment is perfused with high-potassium solution that destroys the barrier properties of the lower part of the cell membrane. The upper compartment is oerfused with normal Ringer solution and the part of the membrane in contact with it demonstrates usual excitability; Replacement of the high-potassium solution in the lower compartment by a potassium-free one abolished the delayed outward current through the working part of the membrane indicating a free acess of ions to and from its inner surfacemthe investigated membrane maintains its excitability for several hours beeing perfused with the F- and PO4--salts of K+ and Tris

摘要

该方法用于对分离的苹果螺神经元进行细胞内灌注。将细胞置于静水压力下,使其进入塑料薄膜上的小孔,该薄膜将实验腔分隔为两个隔室。下隔室用高钾溶液灌注,这会破坏细胞膜下部的屏障特性。上隔室用正常林格溶液灌注,与之接触的那部分膜表现出正常的兴奋性;用无钾溶液替换下隔室中的高钾溶液,消除了通过膜工作部分的延迟外向电流,这表明离子可以自由进出其内表面。在用钾离子和三羟甲基氨基甲烷的氟化物和磷酸盐灌注时,所研究的膜能保持其兴奋性达数小时。

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