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通过结晶脱盐:利用质谱法检测皮升缓冲液中的阿托摩尔生物分子。

Desalting by crystallization: detection of attomole biomolecules in picoliter buffers by mass spectrometry.

作者信息

Gong Xiaoyun, Xiong Xingchuang, Wang Song, Li Yanyan, Zhang Sichun, Fang Xiang, Zhang Xinrong

机构信息

Beijing Key Laboratory for Microanalytical Methods and Instrumentation, Department of Chemistry, Tsinghua University , Beijing 100084, China.

National Institute of Metrology , Beijing 100013, China.

出版信息

Anal Chem. 2015 Oct 6;87(19):9745-51. doi: 10.1021/acs.analchem.5b01877. Epub 2015 Sep 8.

Abstract

Sensitive detection of biomolecules in small-volume samples by mass spectrometry is, in many cases, challenging because of the use of buffers to maintain the biological activities of proteins and cells. Here, we report a highly effective desalting method for picoliter samples. It was based on the spontaneous separation of biomolecules from salts during crystallization of the salts. After desalting, the biomolecules were deposited in the tip of the quartz pipet because of the evaporation of the solvent. Subsequent detection of the separated biomolecules was achieved using solvent assisted electric field induced desorption/ionization (SAEFIDI) coupled with mass spectrometry. It allowed for direct desorption/ionization of the biomolecules in situ from the tip of the pipet. The organic component in the assistant solvent inhibited the desorption/ionization of salts, thus assured successful detection of biomolecules. Proteins and peptides down to 50 amol were successfully detected using our method even if there were 3 × 10(5) folds more amount of salts in the sample. The concentration and ion species of the salts had little influence on the detection results.

摘要

在许多情况下,由于使用缓冲液来维持蛋白质和细胞的生物活性,通过质谱法对小体积样品中的生物分子进行灵敏检测具有挑战性。在此,我们报告了一种针对皮升样品的高效脱盐方法。它基于盐结晶过程中生物分子与盐的自发分离。脱盐后,由于溶剂蒸发,生物分子沉积在石英移液管尖端。随后,使用溶剂辅助电场诱导解吸/电离(SAEFIDI)与质谱联用对分离出的生物分子进行检测。它允许生物分子从移液管尖端原位直接解吸/电离。辅助溶剂中的有机成分抑制了盐的解吸/电离,从而确保了生物分子的成功检测。即使样品中的盐含量高出3×10⁵倍,使用我们的方法仍成功检测到了低至50 amol的蛋白质和肽。盐的浓度和离子种类对检测结果影响很小。

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