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电喷雾液滴撞击/二次离子质谱的基本方面。

Fundamental aspects of electrospray droplet impact/SIMS.

作者信息

Hiraoka Kenzo, Mori Kunihiko, Asakawa Daiki

机构信息

Clean Energy Research Center, University of Yamanashi, Takeda-4, Kofu 400-8510, Japan.

出版信息

J Mass Spectrom. 2006 Jul;41(7):894-902. doi: 10.1002/jms.1048.

DOI:10.1002/jms.1048
PMID:16770831
Abstract

A new ionization method, electrospray droplet impact ionization (EDI), has been developed for matrix-free secondary-ion mass spectrometry (SIMS). The charged droplets formed by electrospraying 1 M acetic acid aqueous solution are sampled through an orifice with a diameter of 400 microm into the first vacuum chamber, transported into a quadrupole ion guide, and accelerated by 10 kV after exiting the ion guide. The droplets impact on a dry solid sample (no matrix used) deposited on a stainless steel substrate. The secondary ions formed by the impact are transported to a second quadrupole ion guide and mass-analyzed by an orthogonal time-of-flight mass spectrometer (TOF-MS). Ten pmol of gramicidin S could be detected with the presence of as much as 10 nmol of NaCl. The ion signal for arginine disappeared with decrease in the substrate temperature below 150 K owing to the formation of ice film over the sample surface. While 10 fmol of gramicidin S could be detected for 30 min, the ionization/desorption efficiency for EDI becomes smaller with an increase in the molecular weight (MW) of a biological sample. The largest protein samples detected to date are cytochrome c and lysozyme. The high sensitivity for EDI is due to the fact that samples only a few monolayers thick are subject to desorption/ionization by EDI, with little fragmentation. A coherent phonon excitation may be the main mechanism for the desorption/ionization of the solid sample.

摘要

一种用于无基质二次离子质谱(SIMS)的新电离方法——电喷雾液滴撞击电离(EDI)已被开发出来。通过电喷雾1M醋酸水溶液形成的带电液滴通过一个直径为400微米的孔被采样到第一个真空室中,传输到四极离子导向器中,并在离开离子导向器后被10kV加速。液滴撞击沉积在不锈钢基底上的干燥固体样品(未使用基质)。撞击产生的二次离子被传输到第二个四极离子导向器,并由正交飞行时间质谱仪(TOF-MS)进行质量分析。在存在多达10nmol氯化钠的情况下,可以检测到10pmol的短杆菌肽S。由于样品表面形成冰膜,当基底温度降至150K以下时,精氨酸的离子信号消失。虽然在30分钟内可以检测到10fmol的短杆菌肽S,但EDI的电离/解吸效率随着生物样品分子量(MW)的增加而变小。迄今为止检测到的最大蛋白质样品是细胞色素c和溶菌酶。EDI的高灵敏度是由于只有几层厚的样品通过EDI进行解吸/电离,且几乎没有碎片化。相干声子激发可能是固体样品解吸/电离的主要机制。

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