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基于薄壁锥形喷口和大体积双样品预浓缩的毛细管电泳-质谱联用技术进行超灵敏单细胞代谢组学分析。

Ultrasensitive Single Cell Metabolomics by Capillary Electrophoresis-Mass Spectrometry with a Thin-Walled Tapered Emitter and Large-Volume Dual Sample Preconcentration.

机构信息

RIKEN Center for Biosystems Dynamics Research , Suita , Osaka 565-0874 , Japan.

Japan Science and Technology Agency , PRESTO, Kawaguchi , Saitama 332-0012 , Japan.

出版信息

Anal Chem. 2019 Aug 20;91(16):10564-10572. doi: 10.1021/acs.analchem.9b01578. Epub 2019 Jul 29.

DOI:10.1021/acs.analchem.9b01578
PMID:31357863
Abstract

Single cell metabolome analysis is essential for studying microscale life phenomena such as neuronal networks and tumor microenvironments. Capillary electrophoresis-mass spectrometry (CE-MS) is one of the most sensitive technologies; however, its sensitivity is still not enough for single cell analysis on general human cells such as HeLa. To address these issues, we first developed an efficient ionization emitter, named as a "nanoCESI" emitter, that had a thin-walled (∼10 μm) and tapered (5-10 μm) end. The thin conductive wall enabled sheathless ionization and minimized the flow rate of ionizing sample, and the tapered end efficiently ionized analytes via an electrospray ionization mechanism, providing up to 3.5-fold increase in sensitivity compared with a conventional sheathless emitter. Fifty repetitive analyses on 20 amino acids were successfully achieved with a nanoCESI emitter. Relative standard deviations of 50 analyses were 1.5%, 4.4%, and 6.8% for migration time, peak height, and peak area, respectively, where a limit of detection (LOD) of 170 pM (850 zmol) was achieved. Second, a sample enrichment method, large-volume dual preconcentration by isotachophoresis and stacking (LDIS), was applied to a newly designed protocol of nanoCESI-MS. This approach achieved up to 380-fold enhanced sensitivity and LOD of 450 fM. Compared with normal sheathless CE-MS, coupling of nanoCESI and LDIS provided up to 800-fold increase of sensitivity in total. Finally, metabolome analyses of single HeLa cells were performed, where 20 amino acids were successfully quantified with triple-quadrupole MS and 40 metabolites were identified with quadrupole-time-of-flight MS, as a promising analytical platform for microscale bioanalysis for the next generation.

摘要

单细胞代谢组分析对于研究神经元网络和肿瘤微环境等微观生命现象至关重要。毛细管电泳-质谱联用技术(CE-MS)是最灵敏的技术之一;然而,其灵敏度对于一般人类细胞(如 HeLa 细胞)的单细胞分析仍然不够。为了解决这些问题,我们首先开发了一种高效的电离发射器,称为“纳米 CESI”发射器,它具有薄壁(约 10 μm)和锥形(5-10 μm)的末端。薄壁使鞘流离子化成为可能,并最小化了离子化样品的流速,而锥形末端则通过电喷雾电离机制有效地将分析物离子化,与传统的无鞘流发射器相比,灵敏度提高了 3.5 倍。使用纳米 CESI 发射器成功地对 20 种氨基酸进行了 50 次重复性分析。50 次分析的迁移时间、峰高和峰面积的相对标准偏差分别为 1.5%、4.4%和 6.8%,检测限(LOD)为 170 pM(850 zmol)。其次,应用大体积双区等速电泳浓缩和堆积(LDIS)的样品富集方法,结合新设计的纳米 CESI-MS 方案。这种方法实现了高达 380 倍的灵敏度增强和 450 fM 的 LOD。与普通无鞘流 CE-MS 相比,纳米 CESI 和 LDIS 的结合提供了高达 800 倍的总灵敏度。最后,对单个 HeLa 细胞的代谢组进行了分析,使用三重四极杆 MS 成功定量了 20 种氨基酸,使用四极杆-飞行时间 MS 鉴定了 40 种代谢物,为下一代微尺度生物分析提供了一种有前途的分析平台。

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