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利用多同位素成像质谱法(MIMS)进行纳米尺度的代谢分析。

Metabolic Analysis at the Nanoscale with Multi-Isotope Imaging Mass Spectrometry (MIMS).

作者信息

Narendra Derek P, Steinhauser Matthew L

机构信息

National Institute of Neurological Disorders and Stroke, National Institutes of Health, Bethesda, Maryland.

Department of Medicine, Aging Institute, University of Pittsburgh School of Medicine, Pittsburgh, Pennsylvania.

出版信息

Curr Protoc Cell Biol. 2020 Sep;88(1):e111. doi: 10.1002/cpcb.111.

DOI:10.1002/cpcb.111
PMID:32706155
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC7484994/
Abstract

Incorporation of a stable-isotope metabolic tracer into cells or tissue can be followed at submicron resolution by multi-isotope imaging mass spectrometry (MIMS), a form of imaging secondary ion microscopy optimized for accurate isotope ratio measurement from microvolumes of sample (as small as ∼30 nm across). In a metabolic MIMS experiment, a cell or animal is metabolically labeled with a tracer containing a stable isotope. Relative accumulation of the heavy isotope in the fixed sample is then measured as an increase over its natural abundance by MIMS. MIMS has been used to measure protein turnover in single organelles, track cellular division in vivo, visualize sphingolipid rafts on the plasma membrane, and measure dopamine incorporation into dense-core vesicles, among other biological applications. In this article, we introduce metabolic analysis using NanoSIMS by focusing on two specific applications: quantifying protein turnover in single organelles of cultured cells and tracking cell replication in mouse tissues in vivo. These examples illustrate the versatility of metabolic analysis with MIMS. © 2020 Wiley Periodicals LLC. Basic Protocol 1: Metabolic labeling for MIMS Basic Protocol 2: Embedding of samples for correlative transmission electron microscopy and MIMS with a genetically encoded reporter Alternate Protocol: Embedding of samples for correlative light microscopy and MIMS Support Protocol: Preparation of silicon wafers as sample supports for MIMS Basic Protocol 3: Analysis of MIMS data.

摘要

通过多同位素成像质谱(MIMS),可以在亚微米分辨率下追踪稳定同位素代谢示踪剂在细胞或组织中的掺入情况。MIMS是一种成像二次离子显微镜,经过优化可从微量样品(直径小至约30纳米)中准确测量同位素比率。在代谢MIMS实验中,细胞或动物用含有稳定同位素的示踪剂进行代谢标记。然后,通过MIMS测量固定样品中重同位素的相对积累量,即相对于其自然丰度的增加量。MIMS已被用于测量单个细胞器中的蛋白质周转、追踪体内细胞分裂、可视化质膜上的鞘脂筏以及测量多巴胺掺入致密核心囊泡等生物学应用。在本文中,我们通过关注两个特定应用来介绍使用纳米二次离子质谱(NanoSIMS)进行的代谢分析:定量培养细胞单个细胞器中的蛋白质周转以及追踪小鼠组织中体内细胞复制。这些例子说明了MIMS代谢分析的多功能性。© 2020威利期刊有限责任公司。基本方案1:MIMS的代谢标记 基本方案2:用于相关透射电子显微镜和带有基因编码报告分子的MIMS的样品包埋 替代方案:用于相关光学显微镜和MIMS的样品包埋 支持方案:制备作为MIMS样品支撑体的硅片 基本方案3:MIMS数据分析。

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