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发展一种新的双模成像方法:荧光显微镜和高分辨率二次离子质谱的结合。

Development of a new bimodal imaging methodology: a combination of fluorescence microscopy and high-resolution secondary ion mass spectrometry.

机构信息

Department of Materials Science, University of Oxford, Oxford, UK.

出版信息

J Microsc. 2010 Oct;240(1):21-31. doi: 10.1111/j.1365-2818.2010.03380.x.

Abstract

In this paper, we present a new experimental methodology to combine mass spectrometry (NanoSIMS) with fluorescence microscopy to provide subcellular information on the location of small molecules in cultured cells. We demonstrate this by comparing the distribution of 5-bromo-2-deoxyuridine in the same cells given by both NanoSIMS analysis and by fluorescence immunohistochemistry. Fiducial markers in the substrates ensured that the images formed by SIMS mapping of bromine ions could be co-registered exactly with images from fluorescence microscopy. The NanoSIMS was shown to faithfully reproduce the information from fluorescence microscopy, but at a much higher spatial resolution. We then show preliminary SIMS images on the distribution of ATN-224, a therapeutic copper chelator for which there is no fluorescent marker, co-registered with conventional Lysotracker and Hoechst stains on the same cells.

摘要

在本文中,我们提出了一种新的实验方法学,将质谱(NanoSIMS)与荧光显微镜相结合,以提供培养细胞中小分子位置的亚细胞信息。我们通过比较 NanoSIMS 分析和荧光免疫组织化学给出的同一细胞中 5-溴-2-脱氧尿苷的分布来证明这一点。底物中的基准标记确保了通过溴离子 SIMS 映射形成的图像可以与荧光显微镜的图像完全配准。NanoSIMS 被证明可以忠实地再现荧光显微镜的信息,但具有更高的空间分辨率。然后,我们展示了初步的 SIMS 图像,显示了没有荧光标记的治疗性铜螯合剂 ATN-224 的分布,该图像与同一细胞上的常规 Lysotracker 和 Hoechst 染色共定位。

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