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使用具有不连续缓冲液的毛细管电泳进行毛细管内富集、蛋白水解和分离:应用于具有中等酸性和碱性等电点的蛋白质。

In-capillary enrichment, proteolysis and separation using capillary electrophoresis with discontinuous buffers: application on proteins with moderately acidic and basic isoelectric points.

作者信息

Nesbitt Chandra A, Yeung Ken K-C

机构信息

Department of Chemistry, The University of Western Ontario, London, Ontario, Canada.

出版信息

Analyst. 2009 Jan;134(1):65-71. doi: 10.1039/b812628c. Epub 2008 Oct 18.

DOI:10.1039/b812628c
PMID:19082176
Abstract

Advances in mass spectrometry and capillary-format separation continue to improve the sensitivity of protein analysis. Of equal importance is the miniaturization of sample pretreatment such as enrichment and proteolysis. In a previous report (Nesbitt et al., Electrophoresis, 2008, 29, 466-474), nanoliter-volume protein enrichment, tryptic digestion, and partial separation was demonstrated in capillary electrophoresis followed by MALDI mass spectral analysis. A discontinuous buffer system, consisting of ammonium (pH 10) and acetate (pH 4), was used to create a pH junction inside the capillary, trapping a protein with a neutral isoelectric point, myoglobin (pI 7.2). Moreover, co-enrichment of myoglobin with trypsin led to an in-capillary digestion. In this paper, the ability of this discontinuous buffer system to perform similar in-capillary sample pretreatment on proteins with moderately acidic and basic pI was studied and reported. Lentil lectin (pI 8.6) and a multi-phosphorylated protein, beta-casein (pI 5.1), were selected as model proteins. In addition to the previously shown tryptic digestion, proteolysis with endoproteinase Asp-N was also performed. Digestion of these acidic and basic pI proteins produced a few peptides with extreme pI values lying outside the trapping range of the discontinuous buffer. An alteration in the peptide trapping procedure was made to accommodate these analytes. Offline MALDI mass spectral analysis confirmed the presence of the expected peptides. The presented miniaturized sample pretreatment methodology was proven to be applicable on proteins with a moderately wide range of pI. Flexibility in the choice of protease was also evident.

摘要

质谱分析和毛细管形式分离技术的进展不断提高蛋白质分析的灵敏度。同样重要的是样品预处理(如富集和蛋白水解)的小型化。在之前的一份报告中(内斯比特等人,《电泳》,2008年,第29卷,第466 - 474页),在毛细管电泳后进行基质辅助激光解吸电离质谱分析,展示了纳升体积的蛋白质富集、胰蛋白酶消化和部分分离。一种由铵(pH 10)和乙酸盐(pH 4)组成的不连续缓冲系统被用于在毛细管内创建一个pH结,捕获具有中性等电点的蛋白质——肌红蛋白(pI 7.2)。此外,肌红蛋白与胰蛋白酶的共富集导致了毛细管内消化。在本文中,研究并报道了这种不连续缓冲系统对具有中等酸性和碱性pI的蛋白质进行类似毛细管内样品预处理的能力。选择扁豆凝集素(pI 8.6)和一种多磷酸化蛋白质β-酪蛋白(pI 5.1)作为模型蛋白质。除了之前展示的胰蛋白酶消化外,还进行了天冬氨酸内肽酶的蛋白水解。这些酸性和碱性pI蛋白质的消化产生了一些具有极端pI值的肽,这些肽不在不连续缓冲系统的捕获范围内。对肽捕获程序进行了改变以适应这些分析物。离线基质辅助激光解吸电离质谱分析证实了预期肽的存在。所提出的小型化样品预处理方法被证明适用于具有中等广泛pI范围的蛋白质。蛋白酶选择的灵活性也很明显。

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