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A fluorescent-based assay for live cell spatially resolved assessment of vesicular monoamine transporter 2-mediated neurotransmitter transport

机译:活细胞基于荧光分析空间分辨囊泡单胺转运2介导的神经递质转运的评估

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摘要

The vesicular monoamine transporter 2 (VMAT2; Slc18a2) packages monoamines into synaptic vesicles. Monoamine homeostasis is highly regulated and dysfunction may play a role in Parkinson’s disease, Huntington’s disease, drug addiction, and neuropsychiatric disorders. The primary function of VMAT2 is to sequester monoamine neurotransmitters into vesicles for subsequent release; it also sequesters toxicants away from cytosolic sites of action. Identification of compounds that modify the action of VMAT2 may be useful as therapeutic agents for preventing or reversing monoamine-related toxicity. Current methods for measuring VMAT2 function are unable to assess uptake in intact cells. Here, we adapted the Neurotransmitter Uptake Assay (Molecular Devices) to develop a measure of VMAT2 function in live whole cells. This assay contains a fluorescent compound, which is transported into cells by the plasma membrane monoamine transporters and has been marketed as a rapid, high-throughput, plate reader based assay for function of these plasma membrane transporters. We demonstrate a modified version of this assay that can be used to visualize and measure transport into vesicles by VMAT2. HEK293 cell lines stably expressing the dopamine transporter and a mCherry-VMAT2 fusion protein were generated. Confocal microscopy confirmed that the fluorescent compound is transported into mCherry-positive compartments. Furthermore, the VMAT2-specific inhibitor tetrabenazine (TBZ) blocks uptake into the mCherry-positive compartment. Confocal images can be analyzed to generate a measure of VMAT2 activity. In summary, we demonstrate a method for spatially resolved analysis of VMAT2-mediated uptake in live intact cells.
机译:凹凸单胺转运蛋白2(VMAT2; SLC18A2)将单胺包装成突触囊泡。单胺稳态是高度监管的,功能障碍可能在帕金森病,亨廷顿氏病,吸毒成瘾和神经精神疾病中起作用。 VMAT2的主要功能是将单胺神经递质隔离成囊泡以供后续释放;它还螯合远离细胞溶质的作用位点的毒性。鉴定改性VMAT2的作用的化合物可用作预防或逆转单胺相关毒性的治疗剂。用于测量VMAT2功能的当前方法无法评估完整细胞中的摄取。在这里,我们适应神经递质摄取测定(分子装置),以在实时细胞中产生VMAT2功能的量度。该测定含有荧光化合物,其通过血浆膜单胺转运蛋白传送到细胞中,并且已作为这些质膜转运蛋白的功能的基于快速的高通量的板式读取器的试验。我们展示了该测定的修改版本,可用于通过VMAT2可视化和测量传输到囊泡。产生稳定表达多巴胺转运蛋白和MCHERRY-VMAT2融合蛋白的HEK293细胞系。共聚焦显微镜证实荧光化合物被输送到MCHerry阳性室中。此外,VMAT2特异性抑制剂四丁嗪(TBZ)阻断吸收到MCHERRY阳性室中。可以分析共聚焦图像以产生VMAT2活动的量度。总之,我们证明了一种用于在活性细胞中对VMAT2介导的摄取的空间分辨分析的方法。

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