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使用基质辅助激光解吸/电离质谱对低至亚皮摩尔水平的凝胶内消化和膜上消化方法进行比较,用于后续的肽和碎片离子质量分析。

Comparison of in-gel and on-membrane digestion methods at low to sub-pmol level for subsequent peptide and fragment-ion mass analysis using matrix-assisted laser-desorption/ionization mass spectrometry.

作者信息

Courchesne P L, Luethy R, Patterson S D

机构信息

Amgen Inc. Thousand Oaks, CA 91320-1789, USA.

出版信息

Electrophoresis. 1997 Mar-Apr;18(3-4):369-81. doi: 10.1002/elps.1150180311.

DOI:10.1002/elps.1150180311
PMID:9150915
Abstract

The success of the mass spectrometric-based approaches for the identification of gel-separated proteins relies upon recovery of peptides, without high levels of ionization-suppressing contaminants, in solvents compatible with the mass spectrometer being employed. We sought to determine whether in-gel or on-membrane digestion provided a significant advantage when low to sub-pmol quantities of gel-separated proteins were analyzed by matrix-assisted laser-desorption/ionization mass spectrometry (MALDI-MS) with respect to the number and size of released peptides. Serial dilutions of five standard proteins of M(r) 17,000 to 97,000 (from 16 pmol to 125 fmol) were electrophoresed and subjected to in-gel digestion (using a microcolumn clean-up protocol, Courchesne, P.L. and Patterson, S. D., BioTechniques, 1997, in press) or on-membrane digestion following blotting to the PVDF-based membranes, Immobilon-P and Immobilon-CD. Peptide maps were able to be obtained for all proteins at the detection limit of each method (Immobilon-P and Immobilon-CD, 0.5 pmol; and in-gel, 125 fmol), and searches of Swiss-Prot or a non-redundant database (> 193000 entries) successfully identified all of the proteins, except beta-casein. Fragment-ion spectra using a curved-field reflector MALDI-MS were obtained from more than one peptide per protein at loads down to 250 fmol (except beta-casein). Using the uninterpreted data, a search of the nonredundant database and a six-way translation of GenBank dbEST (> 2,208,000 entries total) was able to identify myoglobin, carbonic anhydrase II, and phosphorylase b.

摘要

基于质谱法鉴定凝胶分离蛋白质的成功,依赖于在与所使用的质谱仪兼容的溶剂中回收肽段,且不存在高水平的电离抑制污染物。我们试图确定,当通过基质辅助激光解吸/电离质谱(MALDI-MS)分析低至亚皮摩尔量的凝胶分离蛋白质时,胶内消化或膜上消化在释放肽段的数量和大小方面是否具有显著优势。对5种相对分子质量为17,000至97,000的标准蛋白质(从16皮摩尔到125飞摩尔)进行系列稀释,然后进行电泳,并在胶内消化(使用微柱净化方案,库尔谢讷,P.L.和帕特森,S.D.,《生物技术》,1997年,即将发表),或在印迹到基于PVDF的膜(Immobilon-P和Immobilon-CD)后进行膜上消化。在每种方法的检测限(Immobilon-P和Immobilon-CD为0.5皮摩尔;胶内为125飞摩尔)下,所有蛋白质都能获得肽图,并且对Swiss-Prot或非冗余数据库(>193000条记录)的搜索成功鉴定了所有蛋白质,但β-酪蛋白除外。使用弯曲场反射器MALDI-MS,在低至250飞摩尔的上样量下,每种蛋白质可从一个以上的肽段获得碎片离子谱(β-酪蛋白除外)。使用未解释的数据,对非冗余数据库进行搜索以及对GenBank dbEST(总共>2,208,000条记录)进行六向翻译,能够鉴定出肌红蛋白、碳酸酐酶II和磷酸化酶b。

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