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基于惯性力辅助的高通量、无液滴、单细胞采样与 ICP-MS 联用的实时细胞分析。

Inertial-Force-Assisted, High-Throughput, Droplet-Free, Single-Cell Sampling Coupled with ICP-MS for Real-Time Cell Analysis.

机构信息

Research Center for Analytical Sciences, Department of Chemistry, College of Sciences, Northeastern University, Shenyang, Liaoning 110819, People's Republic of China.

出版信息

Anal Chem. 2020 May 5;92(9):6604-6612. doi: 10.1021/acs.analchem.0c00376. Epub 2020 Apr 13.

DOI:10.1021/acs.analchem.0c00376
PMID:32233376
Abstract

Single-cell analysis facilitates perception into the most essential processes in life's mysteries. While it is highly challenging to quantify them at the single-cell level, where precise single-cell sampling is the prerequisite. Herein, a real-time single-cell quantitative platform was established for high-throughput droplet-free single-cell sampling into time-resolved (TRA) ICP-MS and real-time quantification of intracellular target elements. The concentrated cells (2 × 10 cells mL) were spontaneously and orderly aligned in a spiral microchannel with 104 periodic dimensional confined micropillars. The quantification is conducted simultaneously by internal standard inducing from another branch channel in the chip. The flow-rate-independent feature of single-cell focusing into an aligned stream within a wide range of fluidic velocities (100-800 μL min) facilitates high-throughput, oil-free, single-cell introduction into TRA-ICP-MS. The system was used for real-time exploration of intracellular antagonism of Cu against Cd. an obvious antagonistic effect was observed for the MCF-7 cell by culturing for 3, 6, 9, and 12 h with 100 μg L Cd and 100 μg L Cu, and a rivalry rate of 12.8% was achieved at 12 h. At identical experimental conditions, however, limited antagonistic effect was encountered for a bEnd3 cell within the same incubation time period, with a rivalry rate of 4.81%. On the contrary, an antagonistic effect was not observed for the HepG2 cell by culturing for 6 h, while an obvious antagonistic effect was found by further culturing to 12 h, with a rivalry rate of 10.43%. For all three cell lines, significant heterogeneity was observed among individual cells.

摘要

单细胞分析有助于深入了解生命奥秘中最基本的过程。虽然在单细胞水平上进行定量分析极具挑战性,但精确的单细胞采样是前提。在此,建立了一种实时单细胞定量平台,用于无液滴高通量单细胞采样进入时间分辨(TRA)ICP-MS,并实时定量细胞内靶元素。浓缩细胞(2×10 个细胞/mL)在具有 104 个周期性尺寸受限微柱的螺旋微通道中自发且有序排列。通过芯片中另一个分支通道内的内标诱导同时进行定量。在广泛的流速范围内(100-800 μL/min),单细胞聚焦到对齐流中的流速独立特性有利于高通量、无油、单细胞引入 TRA-ICP-MS。该系统用于实时探索铜对镉的细胞内拮抗作用。通过用 100 μg/L Cd 和 100 μg/L Cu 培养 MCF-7 细胞 3、6、9 和 12 h,观察到明显的拮抗作用,在 12 h 时达到 12.8%的竞争率。然而,在相同的实验条件下,对于 bEnd3 细胞,在相同的孵育时间内,拮抗作用有限,竞争率为 4.81%。相反,HepG2 细胞在培养 6 h 时没有观察到拮抗作用,而进一步培养至 12 h 时发现明显的拮抗作用,竞争率为 10.43%。对于所有三种细胞系,个体细胞之间都观察到显著的异质性。

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