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本文引用的文献

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Binding States of Protein-Metal Complexes in Cells.细胞中蛋白质-金属复合物的结合态。
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Electrochemical fecal pellet sensor for simultaneous real-time ex vivo detection of colonic serotonin signalling and motility.用于同时实时离体检测结肠5-羟色胺信号传导和运动的电化学粪便颗粒传感器。
Sci Rep. 2016 Mar 22;6:23442. doi: 10.1038/srep23442.
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Physical connections between different SSVEP neural networks.不同稳态视觉诱发电位神经网络之间的物理连接。
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Highly multiplexed simultaneous detection of RNAs and proteins in single cells.单细胞中RNA和蛋白质的高度多重同步检测。
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Single-cell genome sequencing: current state of the science.单细胞基因组测序:科学现状。
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Label-free cell cycle analysis for high-throughput imaging flow cytometry.用于高通量成像流式细胞术的无标记细胞周期分析
Nat Commun. 2016 Jan 7;7:10256. doi: 10.1038/ncomms10256.
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Adult mouse cortical cell taxonomy revealed by single cell transcriptomics.单细胞转录组学揭示成年小鼠皮质细胞分类学
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Electrophysiological, transcriptomic and morphologic profiling of single neurons using Patch-seq.使用Patch-seq对单个神经元进行电生理、转录组和形态学分析。
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Highly multiplexed imaging of single cells using a high-throughput cyclic immunofluorescence method.使用高通量循环免疫荧光法对单细胞进行高度多重成像。
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A flow cytometry-based method to simplify the analysis and quantification of protein association to chromatin in mammalian cells.一种基于流式细胞术的方法,用于简化对哺乳动物细胞中蛋白质与染色质结合的分析和定量。
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使用质谱法对化学成分、生理变化和代谢进行单神经元识别。

Single-neuron identification of chemical constituents, physiological changes, and metabolism using mass spectrometry.

作者信息

Zhu Hongying, Zou Guichang, Wang Ning, Zhuang Meihui, Xiong Wei, Huang Guangming

机构信息

CAS Key Laboratory of Urban Pollutant Conversion, School of Chemistry and Materials Science, University of Science and Technology of China, Hefei, Anhui 230026, China.

School of Life Sciences, University of Science and Technology of China, Hefei 230026, China.

出版信息

Proc Natl Acad Sci U S A. 2017 Mar 7;114(10):2586-2591. doi: 10.1073/pnas.1615557114. Epub 2017 Feb 21.

DOI:10.1073/pnas.1615557114
PMID:28223513
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC5347563/
Abstract

The use of single-cell assays has emerged as a cutting-edge technique during the past decade. Although single-cell mass spectrometry (MS) has recently achieved remarkable results, deep biological insights have not yet been obtained, probably because of various technical issues, including the unavoidable use of matrices, the inability to maintain cell viability, low throughput because of sample pretreatment, and the lack of recordings of cell physiological activities from the same cell. In this study, we describe a patch clamp/MS-based platform that enables the sensitive, rapid, and in situ chemical profiling of single living neurons. This approach integrates modified patch clamp technique and modified MS measurements to directly collect and detect nanoliter-scale samples from the cytoplasm of single neurons in mice brain slices. Abundant possible cytoplasmic constituents were detected in a single neuron at a relatively fast rate, and over 50 metabolites were identified in this study. The advantages of direct, rapid, and in situ sampling and analysis enabled us to measure the biological activities of the cytoplasmic constituents in a single neuron, including comparing neuron types by cytoplasmic chemical constituents; observing changes in constituent concentrations as the physiological conditions, such as age, vary; and identifying the metabolic pathways of small molecules.

摘要

在过去十年中,单细胞分析技术已成为一项前沿技术。尽管单细胞质谱(MS)最近取得了显著成果,但尚未获得深入的生物学见解,这可能是由于各种技术问题,包括不可避免地使用基质、无法维持细胞活力、由于样品预处理导致的低通量以及缺乏对同一细胞的细胞生理活动记录。在本研究中,我们描述了一种基于膜片钳/质谱的平台,该平台能够对单个活神经元进行灵敏、快速和原位化学分析。这种方法整合了改进的膜片钳技术和改进的质谱测量,以直接从小鼠脑片单个神经元的细胞质中收集和检测纳升规模的样品。在单个神经元中以相对较快的速度检测到了大量可能的细胞质成分,并且在本研究中鉴定出了50多种代谢物。直接、快速和原位采样与分析的优势使我们能够测量单个神经元中细胞质成分的生物学活性,包括通过细胞质化学成分比较神经元类型;观察随着年龄等生理条件变化时成分浓度的变化;以及鉴定小分子的代谢途径。