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Automated mass spectrometry imaging of over 2000 proteins from tissue sections at 100-μm spatial resolution

机译:从2000多个蛋白质的自动质谱成像从组织切片处以100μm空间分辨率

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摘要

Biological tissues exhibit complex spatial heterogeneity that directs the functions of multicellular organisms. Quantifying protein expression is essential for elucidating processes within complex biological assemblies. Imaging mass spectrometry (IMS) is a powerful emerging tool for mapping the spatial distribution of metabolites and lipids across tissue surfaces, but technical challenges have limited the application of IMS to the analysis of proteomes. Methods for probing the spatial distribution of the proteome have generally relied on the use of labels and/or antibodies, which limits multiplexing and requires a priori knowledge of protein targets. Past efforts to make spatially resolved proteome measurements across tissues have had limited spatial resolution and proteome coverage and have relied on manual workflows. Here, we demonstrate an automated approach to imaging that utilizes label-free nanoproteomics to analyze tissue voxels, generating quantitative cell-type-specific images for 2000 proteins with 100-μm spatial resolution across mouse uterine tissue sections preparing for blastocyst implantation.
机译:生物组织表现出络合的空间异质性,其引导多细胞生物的功能。定量蛋白表达对于阐明复杂生物组合物中的方法是必不可少的。成像质谱(IMS)是一种强大的新出现工具,用于将代谢物和脂质的空间分布划过组织表面,但技术挑战限制了IMS对蛋白质素分析的应用。探测蛋白质组的空间分布的方法通常依赖于使用标签和/或抗体,这限制了多路复用并且需要先验的蛋白质目标知识。过去在组织中进行空间解决的蛋白质组测量的过去的努力已经有限的空间分辨率和蛋白质组覆盖,并且依赖于手动工作流程。在这里,我们证明了一种自动成像的成像方法,其利用无标记的纳米蛋白组来分析组织体素,以跨小鼠子宫组织切片在制备胚泡植入的小鼠子宫组织切片上产生数量细胞类型特异性图像。

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