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用于单细胞化学分析的分段光阱毛细管电泳激光诱导天然荧光系统。

A hyphenated optical trap capillary electrophoresis laser induced native fluorescence system for single-cell chemical analysis.

机构信息

Department of Chemistry, University of Illinois at Urbana-Champaign, Urbana, IL 61801, USA.

出版信息

Analyst. 2012 Jul 7;137(13):2965-72. doi: 10.1039/c2an35198f. Epub 2012 Apr 30.

Abstract

Single-cell measurements allow a unique glimpse into cell-to-cell heterogeneity; even small changes in selected cells can have a profound impact on an organism's physiology. Here an integrated approach to single-cell chemical sampling and assay are described. Capillary electrophoresis (CE) with laser-induced native fluorescence (LINF) has the sensitivity to characterize natively fluorescent indoles and catechols within individual cells. While the separation and detection approaches are well established, the sampling and injection of individually selected cells requires new approaches. We describe an optimized system that interfaces a single-beam optical trap with CE and multichannel LINF detection. A cell is localized within the trap and then the capillary inlet is positioned near the cell using a computer-controlled micromanipulator. Hydrodynamic injection allows cell lysis to occur within the capillary inlet, followed by the CE separation and LINF detection. The use of multiple emission wavelengths allows improved analyte identification based on differences in analyte fluorescence emission profiles and migration time. The system enables injections of individual rat pinealocytes and quantification of their endogenous indoles, including serotonin, N-acetyl-serotonin, 5-hydroxyindole-3-acetic acid, tryptophol and others. The amounts detected in individual cells incubated in 5-hydroxytryptophan ranged from 10(-14) mol to 10(-16) mol, an order of magnitude higher than observed in untreated pinealocytes.

摘要

单细胞测量可以让我们独特地观察到细胞间的异质性;即使是选定细胞中的微小变化也可能对生物体的生理学产生深远的影响。这里描述了一种单细胞化学采样和分析的综合方法。毛细管电泳(CE)与激光诱导的天然荧光(LINF)具有足够的灵敏度来描述单个细胞内天然荧光吲哚和儿茶酚。虽然分离和检测方法已经成熟,但单个选定细胞的采样和注入需要新的方法。我们描述了一种优化的系统,该系统将单光束光阱与 CE 和多通道 LINF 检测相连接。细胞在陷阱中被定位,然后使用计算机控制的微操作器将毛细管入口定位在细胞附近。通过流体动力学注入,细胞裂解发生在毛细管入口内,随后进行 CE 分离和 LINF 检测。使用多个发射波长可以根据分析物荧光发射轮廓和迁移时间的差异来提高分析物的识别能力。该系统能够对单个大鼠松果体细胞进行注射,并定量分析其内源性吲哚,包括血清素、N-乙酰血清素、5-羟色氨酸-3-乙酸、色醇等。在 5-羟色氨酸孵育的单个细胞中检测到的量从 10(-14) mol 到 10(-16) mol 不等,比未处理的松果体细胞中的观察值高一个数量级。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/bcef/3558031/14862f29908f/nihms435130f1.jpg

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