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对电生理特性明确的单个神经元进行跨膜染料标记和免疫组织化学染色。

Transmembrane dye labeling and immunohistochemical staining of electrophysiologically characterized single neurons.

作者信息

Puche Adam C, Heyward Philip, Shipley Michael T

机构信息

Department of Anatomy and Neurobiology, Program in Neuroscience, School of Medicine, The University of Maryland, Rm. 222, 685 West Baltimore St., Baltimore, MD 21201, USA.

出版信息

J Neurosci Methods. 2004 Aug 30;137(2):235-40. doi: 10.1016/j.jneumeth.2004.02.032.

Abstract

Numerous studies have used whole-cell patch recording to characterize the electrophysiology of neurons and, via intracellular dye filling, the detailed morphology of the same cells. However, it has been difficult to demonstrate the presence of small soluble molecules within such cells, because washout of the soluble contents of the cell into the patch pipette precludes their later detection by immunohistochemistry. This leaves a major gap in our understanding of circuits made up of neurochemically heterogeneous neurons. To bridge this gap we have developed a transmembrane labeling approach, employing membrane-permeant dye in conjunction with perforated patch electrophysiology. Using this method we have successfully recorded from juxtaglomerular cells in the olfactory bulb, reconstructed the morphology of the cells, and demonstrated expression of soluble neurochemical markers within the same cells. This new technique provides a reliable means to link the physiology, morphology, and neurochemistry of single identified neurons studied using patch-clamp recording.

摘要

许多研究已使用全细胞膜片钳记录来表征神经元的电生理学特性,并通过细胞内染料填充来观察相同细胞的详细形态。然而,要证明此类细胞内存在小的可溶性分子一直很困难,因为细胞内的可溶性成分会被冲洗到膜片钳吸管中,从而无法通过免疫组织化学在之后对其进行检测。这使得我们在理解由神经化学性质异质的神经元组成的神经回路方面存在重大空白。为了填补这一空白,我们开发了一种跨膜标记方法,将膜通透性染料与穿孔膜片钳电生理学结合使用。利用这种方法,我们成功地从嗅球中的近肾小球细胞进行了记录,重建了细胞形态,并证明了相同细胞内可溶性神经化学标记物的表达。这项新技术提供了一种可靠的方法,可将使用膜片钳记录研究的单个已鉴定神经元的生理学、形态学和神经化学联系起来。

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