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Spatial profiling with MALDI MS: Distribution of neuropeptides within single neurons

机译:MALDI MS的空间谱分析:单个神经元内神经肽的分布

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MALDI MS imaging and single-cell profiling are important new capabilities for mass spectrometry. The distribution of neuropeptides within a cell plays an important role in the functioning of the cells in a neuronal network. Protocols for subcellular MALDI MS are described that allow comparative peptide profiling of cell bodies and the neuronal processes (neurites) using single isolated neurons from the neuronal model Aplysia californica. The seawater surrounding the neurons is problematic for mass spectrometry and so must be removed in a manner that does not cause morphological changes or a redistribution of the neuropeptides. Several protocols have been investigated for subcellular spatial profiling, including the use of air-drying, replacement of the seawater with deionized water, and substitution of the cell matrix with fluorinert, mineral oil and glycerol, as well as paraformaldehyde fixation. Glycerol stabilization offers the best combination of preservation of cell morphology and prevention of neuropeptide redistribution. The profiles of the peptides in specific neuronal processes and the cell bodies demonstrate a variety of differences that appear to be cell-specific. These methods are suitable for smaller cells and subcellular MS imaging. [References: 45]
机译:MALDI MS成像和单细胞分析是质谱的重要新功能。细胞内神经肽的分布在神经元网络中的细胞功能中起重要作用。描述了用于亚细胞MALDI MS的方案,该方案允许使用来自加州神经ly模型的单个分离的神经元对细胞体和神经元过程(神经突)进行比较肽谱分析。神经元周围的海水对于质谱分析是有问题的,因此必须以不引起神经肽的形态变化或重新分布的方式除去。已经研究了几种用于亚细胞空间分析的方案,包括风干,用去离子水代替海水,用氟代,矿物油和甘油代替细胞基质以及低聚甲醛固定。甘油稳定化提供了保留细胞形态和防止神经肽重新分布的最佳组合。特定神经元过程和细胞体中的肽谱显示出多种差异,这些差异似乎是细胞特异性的。这些方法适用于较小的细胞和亚细胞MS成像。 [参考:45]

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