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用于肽质量指纹图谱分析的多孔硅胶和氧化铝上的激光解吸/电离质谱法。

Laser desorption/ionization mass spectrometry on porous silica and alumina for peptide mass fingerprinting.

作者信息

Shenar Nawar, Martinez Jean, Enjalbal Christine

机构信息

Institut des Biomolécules Max Mousseron, UMR 5247 CNRS-Universités Montpellier 1 et 2, Université Montpellier 2, Montpellier, France.

出版信息

J Am Soc Mass Spectrom. 2008 May;19(5):632-44. doi: 10.1016/j.jasms.2008.02.006. Epub 2008 Mar 4.

Abstract

We investigated a variant of desorption/ionization on porous silicon (DIOS) mass spectrometry utilizing an aqueous suspension of either porous silica gel or porous alumina (pore size of 60 and 90 A, respectively). Laser desorption/ionization (LDI) from samples directly deposited on a stainless steel surface without any inorganic substrates was also achieved. Synthetic peptides designed to cover large sequence diversity constituted our model compounds. Sample preparation, including material conditioning, peptide solubilization, and deposition protocol onto standard matrix-assisted laser desorption/ionization (MALDI) probe, as well as ionization source tuning were optimized to perform sensitive reproducible LDI analyses. The addition of either a cationizing agent or an alkali metal scavenger to the sample suspension allowed modification of the ionization output. Comparing hydrophilic silica gel to hydrophobic reversed-phase silica gel as well as increasing material pore size provided further insights into desorption/ionization processes. Furthermore, mixtures of peptides were analyzed to probe the spectral suppression phenomenon when no interfering organic matrix was present. The results gathered from synthetic peptide cocktails indicated that LDI mass spectrometry on silica gel or alumina constitutes a promising complementary method to MALDI in proteomics for peptide mass fingerprinting.

摘要

我们研究了一种多孔硅解吸/电离(DIOS)质谱的变体,该变体使用多孔硅胶或多孔氧化铝的水悬浮液(孔径分别为60和90埃)。还实现了直接沉积在不锈钢表面而无需任何无机基质的样品的激光解吸/电离(LDI)。设计用于涵盖较大序列多样性的合成肽构成了我们的模型化合物。优化了样品制备过程,包括材料预处理、肽溶解、在标准基质辅助激光解吸/电离(MALDI)探头上的沉积方案以及电离源调谐,以进行灵敏且可重复的LDI分析。向样品悬浮液中添加阳离子化剂或碱金属清除剂可改变电离输出。将亲水性硅胶与疏水性反相硅胶进行比较,以及增加材料孔径,为解吸/电离过程提供了进一步的见解。此外,分析了肽混合物,以探究不存在干扰性有机基质时的光谱抑制现象。从合成肽混合物中收集的结果表明,硅胶或氧化铝上的LDI质谱在蛋白质组学中构成了一种有前景的与MALDI互补的肽质量指纹分析方法。

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