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使用电压敏感染料记录人类肌间神经元。

Recordings from human myenteric neurons using voltage-sensitive dyes.

机构信息

Human Biology, Technische Universität München, Liesel-Beckmann-Strasse 4, 85354 Freising-Weihenstephan, Germany.

出版信息

J Neurosci Methods. 2010 Oct 15;192(2):240-8. doi: 10.1016/j.jneumeth.2010.07.038. Epub 2010 Aug 5.

Abstract

Voltage-sensitive dye (VSD) imaging became a powerful tool to detect neural activity in the enteric nervous system, including its routine use in submucous neurons in freshly dissected human tissue. However, VSD imaging of human myenteric neurons remained a challenge because of limited visibility of the ganglia and dye accessibility. We describe a protocol to apply VSD for recordings of human myenteric neurons in freshly dissected tissue and myenteric neurons in primary cultures. VSD imaging of guinea-pig myenteric neurons was used for reference. Electrical stimulation of interganglionic fiber tracts and exogenous application of nicotine or elevated KCl solution was used to evoke action potentials. Bath application of the VSDs Annine-6Plus, Di-4-ANEPPS, Di-8-ANEPPQ, Di-4-ANEPPDHQ or Di-8-ANEPPS revealed no neural signals in human tissue although most of these VSD worked in guinea-pig tissue. Unlike methylene blue and FM1-43, 4-Di-2-ASP did not influence spike discharge and was used in human tissue to visualize myenteric ganglia as a prerequisite for targeted intraganglionic VSD application. Of all VSDs, only intraganglionic injection of Di-8-ANEPPS by a volume controlled injector revealed neuronal signals in human tissue. Signal-to-noise ratio increased by addition of dipicrylamine to Di-8-ANEPPS (0.98±0.16 vs. 2.4±0.62). Establishing VSD imaging in primary cultures of human myenteric neurons led to a further improvement of signal-to-noise ratio. This allowed us to routinely record spike discharge after nicotine application. The described protocol enabled reliable VSD recordings from human myenteric neurons but may also be relevant for the use of other fluorescent dyes in human tissues.

摘要

电压敏感染料(VSD)成像已成为检测肠神经系统神经活动的有力工具,包括在新鲜解剖的人类组织中的黏膜下神经元中常规使用。然而,由于神经节的可见度有限和染料可及性,人类肌间神经元的 VSD 成像仍然是一个挑战。我们描述了一种应用 VSD 记录新鲜解剖组织中人类肌间神经元和原代培养的肌间神经元的方案。豚鼠肌间神经元的 VSD 成像被用作参考。通过电刺激神经节间纤维束和外源性应用烟碱或升高的 KCl 溶液来诱发动作电位。尽管大多数这些 VSD 在豚鼠组织中有效,但 Annine-6Plus、Di-4-ANEPPS、Di-8-ANEPPQ、Di-4-ANEPPDHQ 或 Di-8-ANEPPS 的 VSD 成像在人类组织中未显示出神经信号。与亚甲蓝和 FM1-43 不同,4-Di-2-ASP 不影响尖峰放电,并且在人类组织中用于可视化肌间神经节,作为靶向神经节内 VSD 应用的前提。在所有 VSD 中,只有通过体积控制注射器向神经节内注射 Di-8-ANEPPS 才能在人类组织中显示神经元信号。添加二吡咯烷到 Di-8-ANEPPS 中可增加信号与噪声比(0.98±0.16 对 2.4±0.62)。在人类肌间神经元的原代培养物中建立 VSD 成像可进一步提高信号与噪声比。这使我们能够在应用烟碱后常规记录尖峰放电。所描述的方案可用于从人类肌间神经元中进行可靠的 VSD 记录,但也可能与人类组织中其他荧光染料的使用有关。

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