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静脉注射伊文思蓝可在原位及解离后标记大鼠视上核的大细胞神经内分泌细胞。

Intravenous injection of Evans Blue labels magnocellular neuroendocrine cells of the rat supraoptic nucleus in situ and after dissociation.

作者信息

Weiss M L, Cobbett P

机构信息

Department of Psychology, Michigan State University, East Lansing 48824-1117.

出版信息

Neuroscience. 1992;48(2):383-95. doi: 10.1016/0306-4522(92)90498-q.

Abstract

Previous work has demonstrated that intravenous injection of neuronal tracers, e.g. horseradish peroxidase or Fast Blue, can retrogradely label neurons in brain areas that project outside the blood-brain barrier, e.g. magnocellular neuroendocrine neurons of the hypothalamus. Here we have shown that 24 h after intravenous injection of the fluorescent retrograde tracer Evans Blue, the same population of magnocellular neuroendocrine neurons is labeled in the paraventricular, supraoptic and accessory magnocellular nuclei. Parvicellular neuroendocrine cells in the paraventricular nuclei are also labeled. Most Evans Blue-labeled magnocellular neuroendocrine cells in the supraoptic nucleus could be stained immunocytochemically for neurophysins, suggesting that these neurons continue to produce their peptide hormones after taking up the fluorescent dye. Ultrastructural observation of supraoptic cells retrogradely labeled with Evans Blue shows that 95% of the neurons appeared healthy. There was no ultrastructural evidence of degeneration, hyperstimulation, or interruption of the axoplasmic flow. Labeling the neuroendocrine cells with Evans Blue did not alter the size of magnocellular cells, the animal's fluid balance or ingestive behavior. Following enzymatic/mechanical dissociation of the supraoptic nucleus from animals that had been injected with Evans Blue 24 h previously, phase-bright neurons that often contained fluorescent material were observed, thus identifying these neurons as neuroendocrine. Recording from identified neuroendocrine cells showed that these neurons generated spontaneous or current-evoked overshooting action potentials with an afterhyperpolarization and had negative resting membrane potentials. Action potential broadening, a feature of magnocellular neurons, was observed during bursts of action potentials elicited by depolarizing current injection. Taken together, this work would suggest that Evans Blue is non-toxic at the doses used and that it provides a method to identify single neuroendocrine cells in primary cell cultures made from adult hypothalamus for voltage-clamp recordings.

摘要

先前的研究表明,静脉注射神经元示踪剂,如辣根过氧化物酶或快蓝,可逆行标记血脑屏障外投射脑区的神经元,如下丘脑的大细胞神经内分泌神经元。在此我们发现,静脉注射荧光逆行示踪剂伊文思蓝24小时后,室旁核、视上核和附属大细胞核中相同群体的大细胞神经内分泌神经元被标记。室旁核中的小细胞神经内分泌细胞也被标记。视上核中大多数伊文思蓝标记的大细胞神经内分泌细胞可通过免疫细胞化学方法进行神经垂体素染色,这表明这些神经元在摄取荧光染料后继续产生其肽类激素。对伊文思蓝逆行标记的视上核细胞进行超微结构观察显示,95%的神经元看起来健康。没有超微结构证据表明存在变性、过度刺激或轴浆流中断。用伊文思蓝标记神经内分泌细胞不会改变大细胞的大小、动物的水平衡或摄食行为。在对24小时前注射过伊文思蓝的动物的视上核进行酶解/机械解离后,观察到了通常含有荧光物质的相位明亮神经元,从而将这些神经元鉴定为神经内分泌神经元。对已鉴定的神经内分泌细胞进行记录表明,这些神经元产生自发或电流诱发的超射动作电位,并伴有后超极化,且静息膜电位为负。在去极化电流注射诱发的动作电位爆发期间,观察到了大细胞神经元特有的动作电位展宽现象。综上所述,这项研究表明,所用剂量的伊文思蓝无毒,并且它提供了一种方法,可用于在由成年下丘脑制成的原代细胞培养物中鉴定单个神经内分泌细胞,以进行电压钳记录。

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