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FM1-43染料在青蛙运动神经末梢中的超微结构定位及其从末梢的释放

FM1-43 dye ultrastructural localization in and release from frog motor nerve terminals.

作者信息

Henkel A W, Lübke J, Betz W J

机构信息

Department of Physiology, University of Colorado Medical School, Denver 80220, USA.

出版信息

Proc Natl Acad Sci U S A. 1996 Mar 5;93(5):1918-23. doi: 10.1073/pnas.93.5.1918.

Abstract

Previous work has shown that the fluorescent styryl dye FM1-43 stains nerve terminals in an activity-dependent fashion. This dye appears to label the membranes of recycled synaptic vesicles by being trapped during endocytosis. Stained terminals can subsequently be destained by repeating nerve stimulation in the absence of dye; the destaining evidently reflects escape of dye into the bathing medium from membranes of exocytosing synaptic vesicles. In the present study we tested two key aspects of this interpretation of FM1-43 behavior, namely: (i) that the dye is localized in synaptic vesicles, and (ii) that it is actually released into the bathing medium during destaining. To accomplish this, we first photolyzed the internalized dye in the presence of diaminobenzidine. This created an electron-dense reaction product that could be visualized in the electron microscope. Reaction product was confined to synaptic vesicles, as predicted. Second, using spectrofluorometry, we quantified the release of dye liberated into the medium from tubocurarine-treated nerve-muscle preparations. Nerve stimulation increased the amount of FM1-43 released, and we estimate that normally a stained synaptic vesicle contains a few hundred molecules of the dye. The key to the successful detection of released FM1-43 was to add the micelle-forming detergent 3-[(3-cholamidopropyl)dimethylammonio]-1-propanesulfonate (CHAPS), which increased FM1-43 quantum yield by more than two orders of magnitude.

摘要

先前的研究表明,荧光苯乙烯基染料FM1-43以一种依赖活性的方式对神经末梢进行染色。这种染料似乎通过在内吞作用期间被困住来标记回收的突触小泡的膜。随后,在没有染料的情况下重复神经刺激,可以使染色的末梢褪色;这种褪色显然反映了染料从胞吐性突触小泡的膜中逸出到浴液中。在本研究中,我们测试了对FM1-43行为的这种解释的两个关键方面,即:(i)染料定位于突触小泡中,以及(ii)在褪色过程中它实际上释放到了浴液中。为了实现这一点,我们首先在二氨基联苯胺存在的情况下对内化的染料进行光解。这产生了一种电子致密的反应产物,可以在电子显微镜下观察到。如预期的那样,反应产物局限于突触小泡中。其次,我们使用荧光分光光度法,对筒箭毒碱处理的神经肌肉标本释放到培养基中的染料进行了定量。神经刺激增加了FM1-43的释放量,并且我们估计正常情况下一个染色的突触小泡含有几百个这种染料分子。成功检测释放的FM1-43的关键是添加形成胶束的去污剂3-[(3-胆酰胺丙基)二甲基铵]-1-丙烷磺酸盐(CHAPS),它使FM1-43的量子产率提高了两个多数量级。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/9482/39883/ac7577b7f6f2/pnas01509-0196-a.jpg

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