Onnerfjord P, Ekström S, Bergquist J, Nilsson J, Laurell T, Marko-Varga G
Department of Analytical Chemistry, Lund University, Sweden.
Rapid Commun Mass Spectrom. 1999;13(5):315-22. doi: 10.1002/(SICI)1097-0231(19990315)13:5<315::AID-RCM483>3.0.CO;2-C.
This work presents a simple method for obtaining homogeneous sample surfaces in matrix-assisted laser desorption/ionisation time-of-flight mass spectrometry (MALDI-TOFMS) for the automated analysis of peptides and proteins. The sample preparation method is based on applying the sample/matrix mixture onto a pre-deposited highly diluted matrix spot. The pre-deposited crystals act as seeds for the new sample containing crystals which become much smaller in size and more evenly distributed than with conventional methods. This 'seed-layer' method was developed, optimised and compared with the dried-droplet method using peptides and proteins in the 1000-20,000 Da range. The seed-layer method increases the surface homogeneity, spot to spot reproducibility and sample washability as compared with the commonly used dried-droplet method. This methodology is applicable to alpha-cyanohydroxycinnamic acid, sinapinic acid and ferulic acid, which all form homogeneous crystal surfaces. Within-spot variation and between-spot variation was investigated using statistics at a 95% confidence level (n = 36). The statistical values were generated from more than 5000 data points collected from 500 spectra. More than 90% of the sample locations results in high intensity spectra with relatively low standard deviations (RSDs). Typically obtained data showed an RSD of 19-35% within a sample spot as well as in-between spots for proteins, and an RSD of < or = 50% for peptides. Linear calibration curves were obtained within one order of magnitude using internal calibration with a point-RSD of 3% (n = 10). The sample homogeneity allows mass spectra (average of 16 laser shots) to be obtained on each individual sample within 15 sec, whereby a 100 spot target plate can be run in 25 min. High density target plates using the seed-layer method were prepared by spotting approximately 100 picoliter droplets onto the target, resulting in sample spots < or = 500 microns in diameter using a flow-through piezo-electric micro-dispenser. By using this automated sample preparation step lower standard deviations are obtained in comparison to manually prepared samples.
本研究提出了一种简单的方法,可在基质辅助激光解吸/电离飞行时间质谱(MALDI-TOFMS)中获得均匀的样品表面,用于肽和蛋白质的自动分析。该样品制备方法是将样品/基质混合物应用于预先沉积的高度稀释的基质斑点上。预先沉积的晶体作为含有晶体的新样品的晶种,这些晶体的尺寸比传统方法小得多且分布更均匀。这种“种子层”方法是针对1000-20,000 Da范围内的肽和蛋白质开发、优化并与干滴法进行比较的。与常用的干滴法相比,种子层方法提高了表面均匀性、斑点间的重现性和样品的可清洗性。该方法适用于α-氰基-4-羟基肉桂酸、芥子酸和阿魏酸,它们都能形成均匀的晶体表面。使用统计学方法在95%置信水平(n = 36)下研究了斑点内变异和斑点间变异。统计值来自从500个光谱收集的5000多个数据点。超过90%的样品位置产生高强度光谱,标准偏差(RSD)相对较低。通常获得的数据显示,蛋白质在样品斑点内以及斑点间的RSD为19-35%,肽的RSD≤50%。使用内部校准在一个数量级内获得线性校准曲线,点RSD为3%(n = 10)。样品的均匀性使得能够在15秒内对每个单独的样品获得质谱(16次激光照射的平均值),从而可以在25分钟内运行100个斑点的靶板。使用种子层方法的高密度靶板是通过将约100皮升液滴点样到靶板上制备的,使用流通式压电微分配器,得到直径≤500微米的样品斑点。与手动制备的样品相比,通过使用这种自动样品制备步骤可获得更低的标准偏差。
Zotero 插件