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使用单克隆抗体对暴露于2,5 -己二醇的大鼠轴突中的细胞骨架变化进行了研究。

Cytoskeletal changes in axons of rats exposed to 2,5-hexanediol, demonstrated using monoclonal antibodies.

作者信息

Bäckström B, Collins V P

出版信息

Neurotoxicology. 1987 Spring;8(1):85-96.

PMID:3561899
Abstract

The changes in axons seen following exposure to 2,5-hexanedione and its metabolites have to date been studied using electron microscopy and conventional silver impregnation techniques. These have their draw-backs and do not identify the molecular components of a pathological change. We have used monoclonal antibodies to neurofilament proteins and tubulin with immunohistochemical techniques. Sprague-Dawley rats were given 2,5-hexanediol in their drinking water. After 2 weeks the rats showed signs of central and peripheral neuropathy, firstly in the hind limbs and this progressed with time of exposure. After 6 weeks, the administration of 2,5-hexanediol was ceased. Many of the rats were by this time paralyzed in the hind limbs. One third of the rats were then sacrificed. The remaining rats were allowed to recover for a 5 or 10 week period. The axonal changes were studied using an indirect immunoperoxidase method with monoclonal antibodies to the neurofilament proteins and tubulin. The injuries were simply, distinctly and reproducibly demonstrated. With this method it was possible to state that the excess material in the axon swellings was formed of neurofilament proteins and not tubulin. New findings such as the grouping of axon swellings in specific areas of cerebral cortex are reported. This report shows the advantage of using immunohistochemical techniques with monoclonal antibodies. These are easily reproducible and dependable methods for demonstrating pathological changes in the neuronal cytoskeleton.

摘要

迄今为止,对于接触2,5 -己二酮及其代谢产物后所观察到的轴突变化,一直是使用电子显微镜和传统的银浸染技术进行研究的。这些方法存在缺陷,无法识别病理变化的分子成分。我们运用免疫组织化学技术,使用了针对神经丝蛋白和微管蛋白的单克隆抗体。给斯普拉格 - 道利大鼠饮用含2,5 -己二醇的水。2周后,大鼠出现中枢和周围神经病变的迹象,首先出现在后肢,且随着接触时间的推移而进展。6周后,停止给予2,5 -己二醇。此时许多大鼠后肢瘫痪。然后处死了三分之一的大鼠。其余大鼠被允许恢复5周或10周。使用针对神经丝蛋白和微管蛋白的单克隆抗体,通过间接免疫过氧化物酶法研究轴突变化。损伤情况得到了简单、清晰且可重复的显示。通过这种方法,可以确定轴突肿胀中的多余物质是由神经丝蛋白而非微管蛋白形成的。报告了一些新发现,如大脑皮质特定区域轴突肿胀的聚集。本报告展示了使用单克隆抗体免疫组织化学技术的优势。这些是用于显示神经元细胞骨架病理变化的易于重复且可靠的方法。

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