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检测和监测神经递质——光谱分析。

Detection and monitoring of neurotransmitters--a spectroscopic analysis.

机构信息

Department of Physics, University of Texas at El Paso, El Paso, TX, USA.

出版信息

Neuromodulation. 2013 May-Jun;16(3):192-9; discussion 198-9. doi: 10.1111/j.1525-1403.2012.00502.x. Epub 2012 Sep 18.

Abstract

OBJECTIVES

We demonstrate that confocal Raman mapping spectroscopy provides rapid, detailed, and accurate neurotransmitter analysis, enabling millisecond time resolution monitoring of biochemical dynamics. As a prototypical demonstration of the power of the method, we present real-time in vitro serotonin, adenosine, and dopamine detection, and dopamine diffusion in an inhomogeneous organic gel, which was used as a substitute for neurologic tissue.

MATERIALS AND METHODS

Dopamine, adenosine, and serotonin were used to prepare neurotransmitter solutions in distilled water. The solutions were applied to the surfaces of glass slides, where they interdiffused. Raman mapping was achieved by detecting nonoverlapping spectral signatures characteristic of the neurotransmitters with an alpha 300 WITec confocal Raman system, using 532 nm neodymium-doped yttrium aluminum garnet laser excitation. Every local Raman spectrum was recorded in milliseconds and complete Raman mapping in a few seconds.

RESULTS

Without damage, dyeing, or preferential sample preparation, confocal Raman mapping provided positive detection of each neurotransmitter, allowing association of the high-resolution spectra with specific microscale image regions. Such information is particularly important for complex, heterogeneous samples, where changes in composition can influence neurotransmission processes. We also report an estimated dopamine diffusion coefficient two orders of magnitude smaller than that calculated by the flow-injection method.

CONCLUSIONS

Accurate nondestructive characterization for real-time detection of neurotransmitters in inhomogeneous environments without the requirement of sample labeling is a key issue in neuroscience. Our work demonstrates the capabilities of Raman spectroscopy in biological applications, possibly providing a new tool for elucidating the mechanism and kinetics of deep brain stimulation.

摘要

目的

我们证明共焦拉曼映射光谱学提供了快速、详细和准确的神经递质分析,能够实现毫秒时间分辨率的生化动力学监测。作为该方法的典型演示,我们实时展示了在体外对血清素、腺苷和多巴胺的检测,以及在非均相有机凝胶中多巴胺的扩散,该凝胶可作为神经组织的替代品。

材料和方法

多巴胺、腺苷和血清素被用于制备蒸馏水中的神经递质溶液。将这些溶液应用于载玻片表面,它们在那里相互扩散。通过使用 WITec alpha 300 共焦拉曼系统检测特征性神经递质的非重叠光谱特征,用 532nm 掺钕钇铝石榴石激光器激发,实现拉曼映射。每一个局部拉曼光谱在毫秒内记录,完整的拉曼映射在几秒钟内完成。

结果

无需损伤、染色或优先制备样品,共焦拉曼映射提供了对每种神经递质的阳性检测,允许将高分辨率光谱与特定的微观图像区域相关联。这种信息对于复杂、不均匀的样本尤其重要,因为组成的变化可能会影响神经传递过程。我们还报告了一个估计的多巴胺扩散系数,比流动注射法计算的扩散系数小两个数量级。

结论

在不均匀环境中实时检测神经递质而无需对样品进行标记的准确非破坏性表征是神经科学中的一个关键问题。我们的工作展示了拉曼光谱在生物应用中的能力,可能为阐明深部脑刺激的机制和动力学提供了一种新工具。

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