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用于质谱分析的在硅片上培养的细胞的制备。

Preparation of cells cultured on silicon wafers for mass spectrometry analysis.

作者信息

Wittig Andrea, Wiemann Martin, Fartmann Michael, Kriegeskotte Christian, Arlinghaus Heinrich F, Zierold Karl, Sauerwein Wolfgang

机构信息

Strahlenklinik, Universität Duisburg-Essen, 45122 Essen, Germany.

出版信息

Microsc Res Tech. 2005 Apr 1;66(5):248-58. doi: 10.1002/jemt.20159.

DOI:10.1002/jemt.20159
PMID:15940684
Abstract

The distribution of specific atoms and molecules within living cells is of high interest in bio-medical research. Laser secondary neutral mass spectrometry (laser-SNMS) and time-of-flight secondary ion mass spectrometry (TOF-SIMS) detect atoms with high sensitivity and spatial resolution. The application of these methods to cultured cells requires special preparation techniques preserving morphological and chemical integrity of the living cells. The cells should, therefore, be grown on a conducting material preventing charging of the sample during ion bombardment. Silicon is currently used as the preferred support material for non-biological samples in mass spectrometry. This study investigates (1) the influence of silicon surfaces on cell growth and (2) the suitability of a sandwiched, rapid freezing method to analyse transmembrane ion gradients. Human melanoma cells were grown on silicon with polished or etched surfaces. Growth kinetics were studied using the Sulforhodamine-B assay. Number, shape, and morphology of the cells were assessed by epifluorescence microscopy of calcein AM- and DAPI-stained cells. Cells were subjected to rapid freezing, freeze-fracturing, and freeze-drying prior to analysis by TOF-SIMS and laser-SNMS. While cell numbers and morphology on the rough silicon wafers were impaired, morphology and growth kinetics of cells on polished silicon were identical to control cells on cell culture tested polystyrene. TOF-SIMS and laser-SNMS resulted in high-resolution elemental images and mass spectra. Measurement of the intracellular Na+ and K+ concentrations revealed a ratio as observed in living cells. In conclusion, culturing cells on polished silicon wafers followed by sandwiched, rapid freezing is an adequate preparation method to study intracellular ion distribution with mass spectrometry.

摘要

活细胞内特定原子和分子的分布在生物医学研究中备受关注。激光二次中性质谱法(laser-SNMS)和飞行时间二次离子质谱法(TOF-SIMS)能够高灵敏度和高空间分辨率地检测原子。将这些方法应用于培养细胞需要特殊的制备技术,以保持活细胞的形态和化学完整性。因此,细胞应生长在导电材料上,以防止离子轰击期间样品带电。目前,硅被用作质谱分析中非生物样品的首选支撑材料。本研究调查了(1)硅表面对细胞生长的影响,以及(2)一种夹心式快速冷冻方法用于分析跨膜离子梯度的适用性。将人黑色素瘤细胞培养在具有抛光或蚀刻表面的硅上。使用磺酰罗丹明-B 测定法研究生长动力学。通过钙黄绿素 AM 和 DAPI 染色细胞的落射荧光显微镜评估细胞的数量、形状和形态。在通过 TOF-SIMS 和 laser-SNMS 分析之前,对细胞进行快速冷冻、冷冻断裂和冷冻干燥。虽然粗糙硅片上的细胞数量和形态受到损害,但抛光硅上细胞的形态和生长动力学与细胞培养测试聚苯乙烯上的对照细胞相同。TOF-SIMS 和 laser-SNMS 产生了高分辨率的元素图像和质谱图。细胞内 Na+和 K+浓度的测量显示出与活细胞中观察到的比例相同。总之,在抛光硅片上培养细胞,然后进行夹心式快速冷冻,是一种用质谱法研究细胞内离子分布的合适制备方法。

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