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用于成像/质谱分析的单细胞制备

Preparation of single cells for imaging/profiling mass spectrometry.

作者信息

Berman Elena S F, Fortson Susan L, Checchi Kyle D, Wu Ligang, Felton James S, Wu Kuang Jen J, Kulp Kristen S

机构信息

Chemistry, Materials, Earth, and Life Sciences Directorate, Lawrence Livermore National Laboratory, 7000 East Avenue, Livermore, CA 94550, USA.

出版信息

J Am Soc Mass Spectrom. 2008 Aug;19(8):1230-6. doi: 10.1016/j.jasms.2008.05.006. Epub 2008 May 17.

DOI:10.1016/j.jasms.2008.05.006
PMID:18565760
Abstract

Characterizing chemical changes within individual cells is important for determining fundamental mechanisms of biological processes that will lead to new biological insights and improved disease understanding. Analyzing biological systems with imaging and profiling mass spectrometry (MS) has gained popularity in recent years as a method for creating chemical maps of biological samples. To obtain mass spectra that provide relevant molecular information about individual cells, samples must be prepared so that salts and other cell culture components are removed from the cell surface and that the cell contents are rendered accessible to the desorption beam. We have designed a cellular preparation protocol for imaging/profiling MS that removes the majority of the interfering species derived from the cellular growth medium, preserves the basic morphology of the cells, and allows chemical profiling of the diffusible elements of the cytosol. Using this method, we are able to reproducibly analyze cells from three diverse cell types: MCF7 human breast cancer cells, Madin-Darby canine kidney (MDCK) cells, and NIH/3T3 mouse fibroblasts. This preparation technique makes possible routine imaging/profiling MS analysis of individual cultured cells, allowing for understanding of molecular processes within individual cells.

摘要

表征单个细胞内的化学变化对于确定生物过程的基本机制非常重要,这将带来新的生物学见解并加深对疾病的理解。近年来,利用成像和质谱分析(MS)对生物系统进行分析作为一种创建生物样品化学图谱的方法越来越受欢迎。为了获得能够提供有关单个细胞相关分子信息的质谱图,必须对样品进行制备,以便从细胞表面去除盐类和其他细胞培养成分,并使细胞内容物能够被解吸束所触及。我们设计了一种用于成像/质谱分析的细胞制备方案,该方案能够去除大部分源自细胞生长培养基的干扰物质,保留细胞的基本形态,并允许对细胞质中的可扩散成分进行化学分析。使用这种方法,我们能够可重复地分析来自三种不同细胞类型的细胞:MCF7人乳腺癌细胞、Madin-Darby犬肾(MDCK)细胞和NIH/3T3小鼠成纤维细胞。这种制备技术使得对单个培养细胞进行常规成像/质谱分析成为可能,有助于了解单个细胞内的分子过程。

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